US5961971A - Biocontrol of fungal soilborne pathogens by Pythium oligandrum - Google Patents

Biocontrol of fungal soilborne pathogens by Pythium oligandrum Download PDF

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US5961971A
US5961971A US08/731,722 US73172296A US5961971A US 5961971 A US5961971 A US 5961971A US 73172296 A US73172296 A US 73172296A US 5961971 A US5961971 A US 5961971A
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Frank N. Martin
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University of Florida
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    • AHUMAN NECESSITIES
    • A01AGRICULTURE; FORESTRY; ANIMAL HUSBANDRY; HUNTING; TRAPPING; FISHING
    • A01NPRESERVATION OF BODIES OF HUMANS OR ANIMALS OR PLANTS OR PARTS THEREOF; BIOCIDES, e.g. AS DISINFECTANTS, AS PESTICIDES OR AS HERBICIDES; PEST REPELLANTS OR ATTRACTANTS; PLANT GROWTH REGULATORS
    • A01N63/00Biocides, pest repellants or attractants, or plant growth regulators containing microorganisms, viruses, microbial fungi, animals or substances produced by, or obtained from, microorganisms, viruses, microbial fungi or animals, e.g. enzymes or fermentates
    • CCHEMISTRY; METALLURGY
    • C07ORGANIC CHEMISTRY
    • C07KPEPTIDES
    • C07K14/00Peptides having more than 20 amino acids; Gastrins; Somatostatins; Melanotropins; Derivatives thereof
    • C07K14/37Peptides having more than 20 amino acids; Gastrins; Somatostatins; Melanotropins; Derivatives thereof from fungi
    • C07K14/375Peptides having more than 20 amino acids; Gastrins; Somatostatins; Melanotropins; Derivatives thereof from fungi from Basidiomycetes
    • CCHEMISTRY; METALLURGY
    • C12BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
    • C12NMICROORGANISMS OR ENZYMES; COMPOSITIONS THEREOF; PROPAGATING, PRESERVING, OR MAINTAINING MICROORGANISMS; MUTATION OR GENETIC ENGINEERING; CULTURE MEDIA
    • C12N1/00Microorganisms, e.g. protozoa; Compositions thereof; Processes of propagating, maintaining or preserving microorganisms or compositions thereof; Processes of preparing or isolating a composition containing a microorganism; Culture media therefor
    • C12N1/14Fungi; Culture media therefor
    • C12N1/145Fungal isolates
    • CCHEMISTRY; METALLURGY
    • C12BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
    • C12RINDEXING SCHEME ASSOCIATED WITH SUBCLASSES C12C - C12Q, RELATING TO MICROORGANISMS
    • C12R2001/00Microorganisms ; Processes using microorganisms
    • C12R2001/645Fungi ; Processes using fungi

Definitions

  • Plant pathogenic Pythium species can kill a plant at the seedling stage or can reduce crop yield by destroying the root system of a mature plant. While diseases in the seedling stage are often controlled by fungicide application, the continued use of certain highly effective fingicides, e.g., metalaxyl, has faced regulatory uncertainty for use in vegetable transplant greenhouse production systems. In addition, continued use of a particular fungicide can result in the development of tolerance by the pathogen. Fumigants such as methyl bromide, which are routinely used on high cash-value crops, also face regulatory uncertainty. Thus, disease control (in particular damping-off) in the production greenhouses as well as in the field following transplanting are a major concern.
  • fingicides e.g., metalaxyl
  • a biological agent that could protect seedlings from disease in the production facility and after transplanting into the field would meet an existing need and provide an advantageous method for controlling disease, e.g., damping off, in agricultural industries.
  • the subject invention concerns novel isolates of P. oligandrum that can be used successfully as a biological control agent capable of protecting crops from disease caused by pathogenic fungal species, including pathogenic Pythium species.
  • the isolates of the subject invention lack pathogenicity on crop plants, have a similar ecology as some pathogenic species, can readily produce inoculum, and are efficacious in controlling disease.
  • Other isolates of this species were found to be associated with soils suppressive to a pathogenic species.
  • biocontrol agent is in the same genus as many of the pathogens that it is capable of controlling, the isolates examined are not pathogenic on any of the crops that have been tested (Drechsler, 1946, Phytopathology 36:781-864; See also Example 7 herein below).
  • Molecular markers to confirm the identification of the biocontrol isolates as P. oligandrum have been identified. See example 6, below.
  • the subject fungus occupies a similar ecological niche as the pathogens and is vegetatively active under similar soil pH, temperature, and moisture regimes. It has an extensive ecological range and has been recovered from a variety of cultivated and noncultivated soils throughout the world. This is an indication of the range of environmental conditions in which it can survive. In addition, such a ubiquitous nature of the subject isolate can ease regulatory concerns regarding the introduction of organisms into areas in which they have not previously been reported.
  • the fungus sporulates readily, and large amounts of oospore inoculum can be produced by either liquid or solid substrate fermentation. These oospore preparations can be capable of prolonged survival for extended periods of time. In vitro experimentation and greenhouse trials suggest that P. oligandrum also can be effective in controlling other soilborne diseases.
  • P. oligandrum Due to similarity in growth conditions in commercial production facilities, and in some cases types of soilless mix used in production, P. oligandrum also can be useful for controlling disease in ornamental container crops.
  • the subject invention also concerns novel methods of production which advantageously result in an efficacious inoculum.
  • the subject invention includes novel nucleotide sequences which can be useful as isolate-specific markers or can be labeled by employing standard procedures or techniques for use as probes. It is well recognized in the art that isolated nucleotide sequences can have other utilities, including non-specific uses that include their use as a molecular weight marker in nucleic acid size determination assays.
  • SEQ ID NO. 1 shows the nucleotide sequence comprising a unique region and flanking regions of an inverted repeat delimited by PstI restriction sites from mitochondrial DNA from Pythium oligandrum isolate 1982-24. A small unique region is present from bases 1278-2649, inclusive.
  • SEQ ID NO. 2 shows the nucleotide sequence comprising a unique region and flanking regions of an inverted repeat delimited by PstI restriction sites from mitochondrial DNA from Pythium oligandrum isolate 1985-5. A small unique region is present from bases 1281-2653, inclusive.
  • SEQ ID NO. 3 shows the nucleotide sequence comprising a unique region and flanking regions of an inverted repeat delimited by PstI restriction sites from mitochondrial DNA from Pythium oligandrum isolate 1986-41. A small unique region is present at bases 1281-2653, inclusive.
  • SEQ ID NO. 4 shows the nucleotide sequence comprising a unique region and flanking regions of an inverted repeat delimited by PstI restriction sites from mitochondrial DNA from Pythium oligaandrum isolate 17-1. A small unique region is present at bases 504-715, inclusive.
  • SEQ ID NO. 5 shows the nucleotide sequence comprising a unique region and flanking regions of an inverted repeat delimited by PstI restriction sites from mitochondrial DNA from Pythium oligandrum isolate 23-5. A small unique region is present at bases 502-684, inclusive.
  • SEQ ID NO. 6 shows the nucleotide sequence comprising a unique region and flanking regions of an inverted repeat delimited by PstI restriction sites from mitochondrial DNA from Pythium oligandrum isolate 1986-42. A small unique region is present at bases 270-664, inclusive.
  • SEQ ID NO. 7 shows the nucleotide sequence comprising a unique region and flanking regions of an inverted repeat delimited by PstI restriction sites from mitochondrial DNA from Pythium oligandrum isolate 27-6.
  • a small unique sequence is present at bases 504 to at least base 565, inclusive.
  • SEQ ID NO. 8 shows the nucleotide sequence comprising a unique region and flanking regions of an inverted repeat delimited by PstI restriction sites from mitochondrial DNA from Pythium oligandrum isolate 30-1.
  • a small unique sequence is present at base 504 to at least base 612, inclusive.
  • FIG. 1 shows linear growth rates of isolates of Pythium oligandrum on corn meal agar for a 24hour period when incubated at the indicated temperatures.
  • the subject invention relates to a novel, efficacious biocontrol agent comprising a nonpathogenic species, Pythium oligandrum.
  • the subject isolate is not pathogenic on plants and shares a similar ecology to the pathogenic species within the same Pythium genus. Therefore, the subject isolates have the advantage of being active under similar environmental conditions and compete for occupation of the same ecological niche as the pathogens.
  • a number of isolates have been evaluated for efficacy in controlling damping-off of tomato transplants. Several isolates have been identified that provided consistent protection from disease in field evaluations over a five-year period.
  • the P. oligandrum of the subject invention are different isolates than the previously-described Pythium species used as biocontrol agents, (e.g., Polygandron described in the aforementioned '317 patent). Another important difference is the different process, e.g., culture medium used to grow the biochemical agent. There is a great deal of variability among isolates, e.g., cultural characteristics (growth rates, response to temperature, spore formation, germination), as well as efficacy in protecting from disease.
  • Morphological characteristics of the isolates conform to the taxonomic characteristics described for the species (Van der Plaats-Niterink, 1981). For isolates grown on liquid grass blade cultures, sporangia are contiguous, forming irregular aggregates consisting of subglobous elements with connecting filamentous parts. Usually formed intercalary but occasionally terminal. Zoospores are produced. Oogonia average 25 ⁇ m in diameter and are covered with conical protuberances 5-7 ⁇ m long and 2-3 ⁇ m at the base. Antheridia are generally lacking. Oospores are aplerotic and average 22 ⁇ m in diameter. Cultural characteristics such as linear growth rates and sporulation may be found in FIG. 1 and Table 1, respectively. Details of molecular characterization of isolates as P. oligandrum may be found in Example 6.
  • Isolates of the subject invention were deposited with the American Type Culture Collection (ATCC), 10801 University Boulevard, Manassas, Va. 20110-2209. The cultures were assigned the following accession numbers by the repository:
  • the subject culture deposits will be stored and made available to the public in accord with the provisions of the Budapest Treaty for the Deposit of Microorganisms, i.e., they will be stored with all the care necessary to keep them viable and uncontaminated for a period of at least five years after the most recent request for the furnishing of a sample of a deposit(s), and in any case, for a period of at least 30 (thirty) years after the date of deposit or for the enforceable life of any patent which may issue disclosing the cultures.
  • the depositor acknowledges the duty to replace the deposit(s) should the depository be unable to furnish a sample when requested, due to the condition of the deposit(s). All restrictions on the availability to the public of the subject culture deposits will be irrevocably removed upon the granting of a patent disclosing them.
  • P. oligandrum can be used for controlling damping-off due to phytopathogenic Pythium spp. in commercial transplant production systems.
  • mtDNA mitochondrial DNA
  • electrophoretic karyotype of chromosomes and nbosomal DNA
  • mtDNA mitochondrial DNA
  • electrophoretic karyotype of chromosomes and nbosomal DNA
  • mtDNA mitochondrial DNA
  • electrophoretic karyotype of chromosomes and nbosomal DNA
  • Recent sequence analysis of the mtDNA has identified regions that are variable among isolates and can be useful for the construction of isolate-specific markers (see SEQ ID. NOs. 1-8). It is understood by those of ordinary skill in the art that such nucleotide sequences can also be useful as molecular weight markers or as probes.
  • Probes can be constructed by labeling the nucleotide sequence of interest with a signal-generating moiety or a component of a signal-generating system using techniques that are well recognized in the art.
  • P. oligandrum of the subject invention is that it is compatible with existing grower practices, including the use of fungicides. Genetically stable mutants of some isolates of the biocontrol agent tolerant to several commonly used fungicides have been developed.
  • the biocontrol agent of the subject invention is used for vegetable transplants. This is due, for example, to the ease with which such agents can be applied: either mixed into the planting medium prior to seeding or drench applied post-planting, techniques that are well-recognized in the art.
  • the soilless mix that is typically used as a growth or potting medium is less biologically complex than field soil. Such soilless mix growth medium can facilitate establishment of the biocontrol agent.
  • the vegetable transplant system has a comparatively small volume of potting medium per seedling that has to be treated. Another advantage of this production system is that the biocontrol agent will be established on the seedlings at the time of transplanting into the field.
  • a single application of the biocontrol agent at the time of planting can protect from disease while the plants are in the production greenhouses as well as when transplanted in the field. Due to similarity in potting medium and greenhouse production systems, the procedure developed for transplant crops also can be useful in ornamental container crops.
  • the subject isolate has been evaluated in the greenhouse for its ability to protect tomato and cucumber transplants from damping-off caused by P. aphanidermatum following planting in field soil.
  • Transplant plugs were infested with a liquid preparation of the biocontrol agent prior to transplanting into field soil naturally infested with phytopathogenic Pythium spp. (primarily P. aphanidermatum, P. ultimum, and P. irregulare).
  • phytopathogenic Pythium spp. primarily P. aphanidermatum, P. ultimum, and P. irregulare.
  • the soils are infested with additional P. aphanidermatum grown in a vermiculite medium. Those isolates that provide a 90% level of control were then tested in the field.
  • the extractable concentrations of Al, Ca, Cu, Fe, K, Mg, Na, P, and Zn were 979.0, 940.0, 0.61, 37.5, 145.0, 145.0, 9.2, 183.0, 4.32 mg/kg soil, respectively.
  • Isolate 70-1 from Florida showed the highest efficacy of all isolates tested. This isolate has provided levels of protection identical to fungicide treatments and allowed for significantly higher stand counts than observed in the untreated controls in seven of the eight trials. Isolates 25-6 and 30-1 (both from the Southwest USA) have also been highly efficacious. Variation in efficacy for isolate 25-6 correlated with seasonal effects, having significantly improved stand count in only 33% of the trials conducted in the fall compared to 75% in the spring. While Rhizoctonia solani was occasionally recovered from diseased seedlings, this was at a low level, and the predominant cause of damping-off were phytopathogenic Pythium spp.
  • isolate 70-1 significantly reduced tomato damping-off, yet P. oligandrum was recovered at a frequency of only 0.1 colonies/cm of root. Even at the time of planting the frequency of recovery on selective medium was not high and was observed primarily on the tap root and crown regions of the seedling.
  • Liquid cultures have been produced on a range of culture media containing readily available substrates such as homogenized vegetable juice.
  • production of oospores for conducting biocontrol trials can be done by growing cultures in a modified clarified V-8 juice broth culture (Ayers and Lumsden, 1975, Phytopathology 65:1094-1100).
  • the medium is prepared by dissolving 1.5 g calcium carbonate in 200 ml of Cambells V-8 juice and pelleting the particulate matter by centrifugation.
  • the supernatant is diluted with deionized water at a rate of 88 ml/l water and amended with cholesterol to a final concentration of 5 ppm.
  • the medium is autoclaved prior to use.
  • Mycelial mats of the cultures are recovered on a sieve after 14 days growth at 25 C., rinsed in sterile water to remove medium and homogenized in a sterile blender. Mature thick walled oospores are counted with a hemacytometer and densities adjusted to desired levels prior to application to transplants. These have been formulated for application either directly to seeds or soil, mixed with a variety of materials for adhesion to seed surfaces, or encapsulated in sodium alginate. Liquid formulations have also been dried for addition to the soil either directly, mixed with kaolin dust, or coated onto perlite. Solid substrate fermentation using a variety of crop seeds also has been evaluated, U.S. Pat. No. 4,259,317.
  • the preferred liquid preparation has been grown in several different media made from industrial byproducts or inexpensive, readily available components.
  • Preferred dry formulations are either liquid fermentation biomass encapsulated in sodium alginate or pulverized dry fermentation products. Preliminary investigations on storage and survivability of inoculum have been conducted; with the dry formulation currently in use, a high level of survival is observed following eight weeks storage at room temperature.
  • Wettable powders are water-dispersable compositions containing the active material, an inert solid extender, and one or more surfactants to provide rapid wetting and to prevent heavy flocculations when suspended in water.
  • the inert extenders which are preferred for use in the wettable powders of this invention containing the active compounds are of mineral or organic origin.
  • Extenders suitable for the wettable powder formulations of this invention are the natural clays, vermiculite, diatomaceous earth, and synthetic mineral fillers derived from silica and silicate. Most preferred filters for this invention are kaolinites, attapulgite clay, montmorillonite clays, synthetic silicas, synthetic magnesium silicate, and calcium sulfate dihydrate. A surface active agent can also be added to give a homogenous and stable formulation.
  • surfactants are the nonionic and anionic types. They are most suitable for the preparation of dry, wettable products of this invention and dispersants. Occasionally a liquid, non-ionic compound which is primarily an emulsifier may serve as both wetter and dispersant.
  • Most preferred wetting agents are alkylbenzene and alkylnaphthalene sulfonates, sulfated fatty alcohols, amines, or acid amides, long chain esters of sodium isethionate, esters of sodium sulfosuccinate, sulfated or sulfonated vegetable oils, and ditertiary acetylenic glycols.
  • Preferred dispersants are methyl cellulose, polyvinyl alcohol, lignin sulfonates, polymeric alkylnaphthalene sulfonates, sodium naphthalene sulfonates, polymethylene bisnaphthalene sulfonate, and sodium-N-methyl-N-(long chain acid) taruates.
  • wetting and dispersing agents in these preferred wettable powder compositions of the invention are usually present at concentrations of from about 0.5 weight percent to 5 weight percent.
  • the inert extender then completes the formulation. Where needed, 0.1 weight percent of the extender may be replaced by a corrosion inhibitor or an anti-foaming agent or both.
  • wettable powder contains a corrosion inhibitor or an anti-foaming agent or both, the corrosion inhibitor should not exceed about 1 percent of the composition, and the anti-foaming agent should not exceed about 0.5 percent by weight of the composition, both replacing equivalent amounts of the inert extender.
  • Dusts are dense powder compositions which are intended for application in dry form. Dusts are characterized by their free-flowing and rapid settling properties so that they are not readily windborne to areas where their presence is not desired. They contain primarily an active ingredient and a dense, free-flowing, solid extender. Their performance is sometimes aided by the inclusion of a wetting agent and convenience in manufacture frequently demands the inclusion of an inert absorptive grinding aid.
  • the wettable powder as described above can also be used in the preparation of dusts. While such wettable powders can be used directly in dust form, it is more advantageous to dilute them by blending with the dense dust diluent. In this manner, dispersing agents, corrosion inhibitors, and anti-foam agents may also be used as components of a dust.
  • the dust compositions of this invention can comprise from about 0.5 to 20.0 weight percent active ingredient, 5 to 25 weight percent filler, 0.0 to 1.0 weight percent wetting agent, and from about 30 to 90 weight percent dense, free-flowing extender, as these terms are used herein.
  • Such dust formulations can contain, in addition, minor amounts of dispersants, corrosion inhibitors, and anti-foam agents derived from the wettable powders used to make the dust.
  • Emulsifiable oils are usually solutions or suspensions of active material in non-water miscible solvents together with a surfactant and/or emulsifier.
  • emulsifiable oil compositions can be made by mixing the active ingredient with an organic solvent and surfactant.
  • Suitable solvents for the compositions of this invention are chlorinated solvents, water immiscible ethers, esters, or ketones alone or in admixture with aromatic hydrocarbons.
  • Suitable surfactants are those ionic or non-ionic agents known to the art as emulsifying agents.
  • Emulsifying agents most suitable for the emulsifiable oil compositions of this invention are long chain alkyl or mercaptan polyethoxy alcohols, alkylaryl polyethoxy alcohols, sorbitan fatty acid esters, polyoxyethylene ethers with sorbitan fatty acid esters, polyethylene glycol esters with fatty rosin acids, fatty alkylol amide condensates, calcium and amine salts of fatty alcohol sulfates, oil soluble petroleum sulfonates, or preferably mixtures of these emulsifying agents should comprise from about 1 to 10 weight percent of the total composition. As described above, however, up to 5 parts of emulsifying agent for each part of active ingredient can be used.
  • emulsifiable oil compositions of the present invention can consist of from about 10 to 50 weight percent active ingredient, about 40 to 82 percent solvents, and about 1 to 10 weight percent emulsifier, as these terms are defined and used above.
  • Granules are physically stable, particulate compositions containing spores and/or mycelia of this invention which adhere to or are distributed through a basic matrix of a coherent, inert carrier with microscopic dimensions.
  • a surfactant can be present in order to aid leaching of the active ingredient from the granule.
  • the inert carrier is preferably of mineral origin, and suitable carriers are natural clays, some pyrophyllites and vermiculite. Suitable wetting agents can be anionic or non-ionic.
  • granule compositions of this invention most suitable carriers are to two types.
  • the first are porous, absorptive pre-formed granules, such as preformed and screened granular attapulgite or heat expanded, granular, screened vermiculite. On either of these, a solution of the active agent can be sprayed and will be absorbed at concentrations up to 25 weight percent of the total weight.
  • the second type are initially powdered kaolin clays, hydrated attapulgite, or bentonite clays in the form of sodium calcium, or magnesium bentonites. Water-soluble salts such as sodium salts may also be present to aid in the disintegrations of the granules in the presence of moisture.
  • ingredients are blended with the active component distributed uniformly throughout the mass.
  • Such granules can also be made with 25 to 30 weight percent active component but more frequently a concentration of about 10 weight percent is desired for optimum distribution.
  • the granular compositions of this invention are believed to be most useful in a size range of 15-30 mesh.
  • wetting agents for the granular compositions of this invention depend upon the type of granule used.
  • the most suitable wetting agents are non-ionic, liquid wetters miscible with the solvent.
  • emulsifiers comprise alkylaryl polyether alcohols, alkyl polyether alcohols, polyoxethylene sorbitan fatty acid esters, polyethylene glycol esters with fatty or rosin acids, fatty alkylol amide condensates, oil petroleum or vegetable oil sulfonates, or mixtures of these.
  • Such agents will usually comprise up to about 5 weight percent of the total composition.
  • liquid non-ionic wetters can still be used, but it is usually preferable to incorporate at the mixing stage one of the solid, powdered anionic wetting agents such as those previously listed for the wettable powders. Such agents should comprise about 0 to 2 percent of the total composition.
  • the preferred granular formulation of this invention comprises about 5 to 30 weight percent active material, about 0 to 5 weight percent wetting agent, and about 65 to 95 percent inert mineral carrier, as these terms are used herein.
  • the mitochondrial DNA is an advantageous molecular marker for use with isolates of genus Pythium.
  • the Pythium mtDNA is highly conserved within a species yet divergent between species to allow differentiation by RFLP analysis of even morphologically similar species.
  • Detailed restriction maps have been constructed for 18 species in the genus and numerous geographically separated isolates of each species to evaluate both inter- as well as intra-specific variation of the genome. This research has supported the validity of using the mitochondrial DNA for taxonomic classification of species in the genus.
  • the isolates used as biocontrol agents described herein have been unequivocally identified as the nonphytopathogenic species P. oligandrum.
  • the mitochondrial genome also has proved to be useful for construction of species, and in some cases isolate specific molecular markers.
  • the organization of the mitochondrial genome in Pythium is unusual in that approximately 80% of the genome is comprised of an inverted repeat.
  • the inverted repeats are separated by two single copy unique regions referred to as the small and large unique region (which is indicative of their relative sizes). It is predominantly in the small unique region where intraspecific variation in restriction maps for this species is observed (Genome 34:156-162).
  • isolate 70-1 has a mtDNA restriction map similar to isolate 82-24.
  • the use of sequences from the small unique region are useful for constructing probes with varying levels of species and isolate specificity (Phytopathology 81:742-746). Subsequent DNA sequence analysis has identified regions of sequence variation which should enhance the prospects for constructing isolate specific probes or PCR primers (See SEQ ID. NOs. 1-8).
  • 1986-42 (SEQ ID NO. 6) has a deletion of 285 bp relative to isolate 17-1 (SEQ ID NO. 4) that removes a portion of the small unique and IR region, causing the IR region to be smaller than 17-1 by 234 bp. This deletion also is observed when comparing 1986-42 (SEQ ID NO. 6) to all other isolates, although the size of the deletion varies.
  • This region contains sequences that are most effective in exhibiting sequence uniqueness (except for 1985-5 SEQ ID NO. 2! and 1986-41 SEQ ID NO. 3!, which are the same). The relative position of this region for each isolate is shown in Table 3.
  • P. oligandrum When coated on seed surfaces, P. oligandrum was found to be nonpathogenic in vitro and in vivo on 12 crop species representing six families (Martin and Hancock, 1987). When planted in fumigated soil, there was no reduction in shoot weight of stand counts. In addition, reduction of root densities was not observed when the plants were grown in field soil. Evaluations of pathogenicity also were conducted with several ornamental crops; none was observed.
  • Pythium oligandrum also has been reported to be nonpathogenic on barley and oats (Kilpatrick, 1968, Plant Dis. Rep. 52:209-212; Bratoloveanu and Wallace, 1982, Biennial Report of the Waite Agricultural Research Institute 85:143 South Australia), pineapple (Klemmer and Nakano, 1964, Plant Dis. Rep. 48:848-852), cress (Al-Hamdani, 1982, Ph.D. dissertation, Dept. of Botany, University of Sheffield; Al-Hamdani et al., 1983, Plant Pathology 32:449-454; Lutchmeah and Cooke, 1984, Trans. Brit. Mycol. Soc.

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Abstract

Described are non-phytopathogenic Pythium oligandrum isolates having activity to control phytopathogenic Pythium spp. or control damping-off of a plant, by applying an effective amount of the non-phytopathogenic isolates to a plant or its situs. The isolates can be applicable crops utilizing transplant systems. Also described are methods of using the isolates and genetic sequences identified from the isolates which can be useful in identification procedures.

Description

BACKGROUND OF THE INVENTION
Within the fungal genus Pythium are plant pathogenic species which can cause significant losses in vegetable production. The value of vegetable crops grown in the state of Florida totaled over $1.79 billion for the 1991-92 crop season with much of the cabbage, cucumber, pepper, and tomato crops planted as transplants. Tomato alone accounts for $735 million in this production total and over 80% of the crop is transplanted. The use of vegetable transplants in commercial field production systems is important in many areas of the United States. In California, all of the celery, fresh market tomato and pepper, and most of the cauliflower and broccoli are grown as transplant crops. In Monterey County alone, the value of the transplants grown in 1992 amounted to nearly $18 million and represented a final crop value of $176 million.
Plant pathogenic Pythium species can kill a plant at the seedling stage or can reduce crop yield by destroying the root system of a mature plant. While diseases in the seedling stage are often controlled by fungicide application, the continued use of certain highly effective fingicides, e.g., metalaxyl, has faced regulatory uncertainty for use in vegetable transplant greenhouse production systems. In addition, continued use of a particular fungicide can result in the development of tolerance by the pathogen. Fumigants such as methyl bromide, which are routinely used on high cash-value crops, also face regulatory uncertainty. Thus, disease control (in particular damping-off) in the production greenhouses as well as in the field following transplanting are a major concern.
In addition to the plant pathogenic species of Pythium, some members of this genus exist strictly as soil saprophytes (Van der Plaats-Niterink, 1981, Monograph of the genus Pythium. Studies in Mycology No. 21. Centraalbureau Voor Schimmelcultures, Baarn, The Netherlands), and several have been identified that are pathogenic on mammals (de Cock et al., 1987, J. Clin. Micro. 25:344-349), fish (Van der Plaats-Niterink, 1981), and insects (Saunders et al, 1988, J. Invert. Path. 52:360-363). One species, Pythium oligandrum Drechsler, is not pathogenic on plants and is effective in protecting plants from attack by pathogenic species.
An alternative to the use of pesticides for controlling phytopathogenic Pythium spp. is the use of biological control agents for vegetable transplants, a large and expanding industry in which disease protection is needed in the greenhouse as well as in the field after transplanting.
U.S. Pat. No. 4,574,083 to Baker and Lifshitz describes Pythium nunn, which is not pathogenic to plants and can protect seedlings from damping-off in greenhouse evaluations. However, P. nunn generally grows slower in culture medium than P. oligandrum but, in contrast to P. oligandrum, can colonize organic substrates in the soil that have already been colonized by other fungi. Pythium nunn also can be difficult to sporulate; sporulation is an essential characteristic for inoculum production. In the soil, P. nunn also behaves differently than P. oligandrum in that, as a primary colonizing saprophyte, it is not as aggressive.
There are a number of studies examining the effect of seed treatment with oospores of P. oligandrum on reducing subsequent levels of disease, most of which have been conducted in the greenhouse. Deacon (1976; Trans. Br. Mycol. Soc. 66:383-391) described the ability of mycelial seed coatings on wheat to significantly reduce the disease incidence over untreated seeds.
Vesely (1977; Phytopath Z. 90:113-115; 1979) observed that application of oospores to sugarbeet seed reduced damping-off incidence to a similar level as thiram treatment (see also Schippers, B. and W. Gams, eds. Academic Press, Soil-Borne Plant Pathogens). In U.S. Pat. No. 4,259,317, Vesely et al describe the application of Pythium oligandrum, or "Polygandron." However, the '317 patent describes a particular isolate P. oligandrum for protecting against damping-off by applying a preparation to sugarbeet seed. There is no description or suggestion in the '317 patent regarding the use of Polygandron on vegetable transplants.
A co-worker and I observed a similar response for disease control when using isolates of P. oligandrum recovered from suppressive soils pelleted onto sugarbeet seeds. See Martin and Hancock (1987; Phytopathology 77:1013-1020). While the emerging radicle was colonized by the biocontrol agent and protected from plant infection, this colonization was limited to association with the seed coat and suggested that the fungus was not rhizosphere competent. Additional greenhouse trials on cress (Al-Hamdani et al, 1983, Plant Pathology 32:449-454; McQuilken et al., 1990 Plant Pathology 39:452-462, 1992 J. Phytopathol 135:125-134); sugarbeet and carrot (Lutchmeah and Cooke, 1985, Plant Pathology 34:528-531); and sugarbeet (Walther and Gindrat, 1987, Journal of Phytopathology 119:167-174) have indicated that seed treatment with P. oligandrum can control other phytopathogenic Pythium spp., Phoma betae, and Mycocentrospora acerina.
A biological agent that could protect seedlings from disease in the production facility and after transplanting into the field would meet an existing need and provide an advantageous method for controlling disease, e.g., damping off, in agricultural industries.
BRIEF SUMMARY OF THE INVENTION
The subject invention concerns novel isolates of P. oligandrum that can be used successfully as a biological control agent capable of protecting crops from disease caused by pathogenic fungal species, including pathogenic Pythium species. Advantageously, the isolates of the subject invention lack pathogenicity on crop plants, have a similar ecology as some pathogenic species, can readily produce inoculum, and are efficacious in controlling disease. Other isolates of this species were found to be associated with soils suppressive to a pathogenic species.
Amendment of field soil naturally infested with phytopathogenic Pythium spp. with oospores of P. oligandrum can also reduce the incidence of disease when cropped to susceptible hosts in the greenhouse (Martin and Hancock, 1987). We have conducted field trials evaluating efficacy in vegetable transplants in Florida and have identified isolates that are as effective as metalaxyl in protecting against phytopathogenic Pythium spp. when added to seedlings prior to transplanting.
It should be emphasized that although the biocontrol agent is in the same genus as many of the pathogens that it is capable of controlling, the isolates examined are not pathogenic on any of the crops that have been tested (Drechsler, 1946, Phytopathology 36:781-864; See also Example 7 herein below). Molecular markers to confirm the identification of the biocontrol isolates as P. oligandrum have been identified. See example 6, below.
Advantageously, the subject fungus occupies a similar ecological niche as the pathogens and is vegetatively active under similar soil pH, temperature, and moisture regimes. It has an extensive ecological range and has been recovered from a variety of cultivated and noncultivated soils throughout the world. This is an indication of the range of environmental conditions in which it can survive. In addition, such a ubiquitous nature of the subject isolate can ease regulatory concerns regarding the introduction of organisms into areas in which they have not previously been reported. The fungus sporulates readily, and large amounts of oospore inoculum can be produced by either liquid or solid substrate fermentation. These oospore preparations can be capable of prolonged survival for extended periods of time. In vitro experimentation and greenhouse trials suggest that P. oligandrum also can be effective in controlling other soilborne diseases.
Due to similarity in growth conditions in commercial production facilities, and in some cases types of soilless mix used in production, P. oligandrum also can be useful for controlling disease in ornamental container crops.
The subject invention also concerns novel methods of production which advantageously result in an efficacious inoculum.
In addition, the subject invention includes novel nucleotide sequences which can be useful as isolate-specific markers or can be labeled by employing standard procedures or techniques for use as probes. It is well recognized in the art that isolated nucleotide sequences can have other utilities, including non-specific uses that include their use as a molecular weight marker in nucleic acid size determination assays.
BRIEF DESCRIPTION OF THE SEQUENCES
SEQ ID NO. 1 shows the nucleotide sequence comprising a unique region and flanking regions of an inverted repeat delimited by PstI restriction sites from mitochondrial DNA from Pythium oligandrum isolate 1982-24. A small unique region is present from bases 1278-2649, inclusive.
SEQ ID NO. 2 shows the nucleotide sequence comprising a unique region and flanking regions of an inverted repeat delimited by PstI restriction sites from mitochondrial DNA from Pythium oligandrum isolate 1985-5. A small unique region is present from bases 1281-2653, inclusive.
SEQ ID NO. 3 shows the nucleotide sequence comprising a unique region and flanking regions of an inverted repeat delimited by PstI restriction sites from mitochondrial DNA from Pythium oligandrum isolate 1986-41. A small unique region is present at bases 1281-2653, inclusive.
SEQ ID NO. 4 shows the nucleotide sequence comprising a unique region and flanking regions of an inverted repeat delimited by PstI restriction sites from mitochondrial DNA from Pythium oligaandrum isolate 17-1. A small unique region is present at bases 504-715, inclusive.
SEQ ID NO. 5 shows the nucleotide sequence comprising a unique region and flanking regions of an inverted repeat delimited by PstI restriction sites from mitochondrial DNA from Pythium oligandrum isolate 23-5. A small unique region is present at bases 502-684, inclusive.
SEQ ID NO. 6 shows the nucleotide sequence comprising a unique region and flanking regions of an inverted repeat delimited by PstI restriction sites from mitochondrial DNA from Pythium oligandrum isolate 1986-42. A small unique region is present at bases 270-664, inclusive.
SEQ ID NO. 7 shows the nucleotide sequence comprising a unique region and flanking regions of an inverted repeat delimited by PstI restriction sites from mitochondrial DNA from Pythium oligandrum isolate 27-6. A small unique sequence is present at bases 504 to at least base 565, inclusive.
SEQ ID NO. 8 shows the nucleotide sequence comprising a unique region and flanking regions of an inverted repeat delimited by PstI restriction sites from mitochondrial DNA from Pythium oligandrum isolate 30-1. A small unique sequence is present at base 504 to at least base 612, inclusive.
BRIEF DESCRIPTION OF THE DRAWINGS
FIG. 1 shows linear growth rates of isolates of Pythium oligandrum on corn meal agar for a 24hour period when incubated at the indicated temperatures.
DETAILED DESCRIPTION OF THE INVENTION
The subject invention relates to a novel, efficacious biocontrol agent comprising a nonpathogenic species, Pythium oligandrum. The subject isolate is not pathogenic on plants and shares a similar ecology to the pathogenic species within the same Pythium genus. Therefore, the subject isolates have the advantage of being active under similar environmental conditions and compete for occupation of the same ecological niche as the pathogens. A number of isolates have been evaluated for efficacy in controlling damping-off of tomato transplants. Several isolates have been identified that provided consistent protection from disease in field evaluations over a five-year period.
The P. oligandrum of the subject invention are different isolates than the previously-described Pythium species used as biocontrol agents, (e.g., Polygandron described in the aforementioned '317 patent). Another important difference is the different process, e.g., culture medium used to grow the biochemical agent. There is a great deal of variability among isolates, e.g., cultural characteristics (growth rates, response to temperature, spore formation, germination), as well as efficacy in protecting from disease.
Morphological characteristics of the isolates conform to the taxonomic characteristics described for the species (Van der Plaats-Niterink, 1981). For isolates grown on liquid grass blade cultures, sporangia are contiguous, forming irregular aggregates consisting of subglobous elements with connecting filamentous parts. Mostly formed intercalary but occasionally terminal. Zoospores are produced. Oogonia average 25 μm in diameter and are covered with conical protuberances 5-7 μm long and 2-3 μm at the base. Antheridia are generally lacking. Oospores are aplerotic and average 22 μm in diameter. Cultural characteristics such as linear growth rates and sporulation may be found in FIG. 1 and Table 1, respectively. Details of molecular characterization of isolates as P. oligandrum may be found in Example 6.
              TABLE 1
______________________________________
Production of sporangia, zoospores, and oospores by select isolates of
Pythium oligandrum with different levels of efficacy in protecting
tomato
transplants from damping-off
Isolate Sporangia.sup.a
                      Zoospores.sup.a
                                Oospores.sup.b
______________________________________
70-1    7.3 B.sup.c   0         66.2 AB
25-6    22.9 E        5         120.1 D
30-1    11.1 C        0         124.9 D
23-5    11.8 CD       15        79.5 BC
48-1    14.6 D        10        54.5 A
24-4    5.5 AB        0         84.9 BC
B-6     7.3 B         0         90.5 C
______________________________________
 .sup.a Sporangia counted in field of view of a stereo microscope at
 95× of isolates grown on grass bladewater cultures that were five
 days old. Zoospore discharge was reduced by placing cultures at 4°
 C. for 30 minutes and allowing to warm up to room temperature.
 .sup.b Oospore counts were made of isolates grown on 1/2 strength V8 juic
 broth for 14 days at 25° C. Values represent average numbers of
 thickwalled mature oospores counted in field of view of compound
 microscope at 200× magnification.
 .sup.c Values in the same column followed by the same letter are not
 significantly different (P = 0.05) as determined by Duncan's multiple
 range test.
Isolates of the subject invention were deposited with the American Type Culture Collection (ATCC), 10801 University Boulevard, Manassas, Va. 20110-2209. The cultures were assigned the following accession numbers by the repository:
______________________________________
Culture       Accession number
                            Deposit date
______________________________________
Pythium oligandrum,
              ATCC 74395    October 8, 1996
isolate 70-1.
Pythium oligandrum,
              ATCC 74393    October 8, 1996
isolate 25-6.
Pythium oligandrum,
              ATCC 74394    October 8, 1996
isolate 30-1.
______________________________________
The subject cultures have been deposited under conditions that assure that access to the culture(s) will be available during the pendency of this patent application to one determined by the Commissioner of Patents and Trademarks to be entitled thereto under 37 CFR 1.14 and 35 USC 122. The deposits are available as required by foreign patent laws in countries wherein counterparts of the subject application, or its progeny, are filed. However, it should be understood that the availability of a deposit does not constitute a license to practice the subject invention in derogation of patent rights granted by governmental action.
Further, the subject culture deposits will be stored and made available to the public in accord with the provisions of the Budapest Treaty for the Deposit of Microorganisms, i.e., they will be stored with all the care necessary to keep them viable and uncontaminated for a period of at least five years after the most recent request for the furnishing of a sample of a deposit(s), and in any case, for a period of at least 30 (thirty) years after the date of deposit or for the enforceable life of any patent which may issue disclosing the cultures. The depositor acknowledges the duty to replace the deposit(s) should the depository be unable to furnish a sample when requested, due to the condition of the deposit(s). All restrictions on the availability to the public of the subject culture deposits will be irrevocably removed upon the granting of a patent disclosing them.
Procedures for the production of efficacious inoculum using inexpensive culture media have been developed, as have methods for inoculum formulation to provide a prolonged shelf life. Preliminary data suggest that this biocontrol agent also is capable of protecting several ornamental container crops from damping-off.
In view of its demonstrated efficacy in field trials, P. oligandrum can be used for controlling damping-off due to phytopathogenic Pythium spp. in commercial transplant production systems.
Evaluations of P. oligandrum as a biological control agent were conducted in Florida. Over 140 isolates have been collected from different geographical regions of the world, many of which have been evaluated for efficacy for protection of transplants in the greenhouse and field (experimentation conducted with APHIS approval and in accordance with their guidelines). Information on the physical and chemical properties of the soils from which many of these isolates were recovered is available. The isolates examined in these investigations have not demonstrated any pathogenicity to the crops tested (a number of different vegetable and grain crops as well as several ornamentals). Extensive molecular genetic characterization of representative isolates also has been done, including analysis of mitochondrial DNA (mtDNA), electrophoretic karyotype of chromosomes, and nbosomal DNA (Genome 34:156-162; Current Genet. 28:255-234; Exp. Mycol. 14:32-46; Phytopathology 81:742-746; Mycologia 87:333-353). Recent sequence analysis of the mtDNA has identified regions that are variable among isolates and can be useful for the construction of isolate-specific markers (see SEQ ID. NOs. 1-8). It is understood by those of ordinary skill in the art that such nucleotide sequences can also be useful as molecular weight markers or as probes. Probes can be constructed by labeling the nucleotide sequence of interest with a signal-generating moiety or a component of a signal-generating system using techniques that are well recognized in the art.
One advantage of the P. oligandrum of the subject invention is that it is compatible with existing grower practices, including the use of fungicides. Genetically stable mutants of some isolates of the biocontrol agent tolerant to several commonly used fungicides have been developed.
In a preferred method, the biocontrol agent of the subject invention is used for vegetable transplants. This is due, for example, to the ease with which such agents can be applied: either mixed into the planting medium prior to seeding or drench applied post-planting, techniques that are well-recognized in the art. In addition, the soilless mix that is typically used as a growth or potting medium is less biologically complex than field soil. Such soilless mix growth medium can facilitate establishment of the biocontrol agent. The vegetable transplant system has a comparatively small volume of potting medium per seedling that has to be treated. Another advantage of this production system is that the biocontrol agent will be established on the seedlings at the time of transplanting into the field. Thus, a single application of the biocontrol agent at the time of planting can protect from disease while the plants are in the production greenhouses as well as when transplanted in the field. Due to similarity in potting medium and greenhouse production systems, the procedure developed for transplant crops also can be useful in ornamental container crops.
Following are examples which illustrate procedures for practicing the invention. These examples should not be construed as limiting. All percentages are by weight and all solvent mixture proportions are by volume unless otherwise noted.
EXAMPLE 1
Greenhouse Screening Trials
The subject isolate has been evaluated in the greenhouse for its ability to protect tomato and cucumber transplants from damping-off caused by P. aphanidermatum following planting in field soil. Transplant plugs were infested with a liquid preparation of the biocontrol agent prior to transplanting into field soil naturally infested with phytopathogenic Pythium spp. (primarily P. aphanidermatum, P. ultimum, and P. irregulare). To ensure that disease levels of untreated controls are between 50-70% seedling death, the soils are infested with additional P. aphanidermatum grown in a vermiculite medium. Those isolates that provide a 90% level of control were then tested in the field.
EXAMPLE 2
Field Trials
Field trials were conducted on a research plot naturally infested with the phytopathogenic species Pythium ultimum, Pythium irregulare, and Pythium aphanidennatum. The population levels were increased to a level which gave approximately 50% death in untreated controls by cropping to susceptible crop varieties and disking under the crop debris. This approach allows for inoculum buildup by pathogenic attack of the host as well as saprophytic buildup through colonization of crop residue. Plots currently have six replicates of 24 plants per treatment. The soil used throughout this investigation was a Chiply sand with 5-10% silt+clay content, 3.72% organic matter, and 238 ppm soluble salts. The native soil pH was 5.3, as determined by measurement of saturation paste after 4 hours incubation. The extractable concentrations of Al, Ca, Cu, Fe, K, Mg, Na, P, and Zn were 979.0, 940.0, 0.61, 37.5, 145.0, 145.0, 9.2, 183.0, 4.32 mg/kg soil, respectively.
Field trials with tomato transplants were conducted for 11 growing seasons with efficacy observed in eight seasons (Table 2); the disease level was high for one season (73% disease in fungicide check) and significant differences among all treatments were not observed in two other seasons.
                                  TABLE 2
__________________________________________________________________________
Summary of plant death observed during eight planting seasons occurring
on tomato
seedlings treated with selected isolates of Pythium oligandrum
% Death
Treatment
     Spring 90
          Fall 90
                Spring 91
                     Spring 92
                          Fall 92
                               Fall 93
                                    Spring 94
                                         Fall 94
__________________________________________________________________________
Untreated
     45.8 B
          47.9 D
                37.5 C
                     33.3 B
                          41.65 B
                               41.1 A
                                    33.3 C
                                         32.6 A
Ridomil
     12.5 AB
           4.0 A
                10.4 AB
                     16.8 AB
                          35.4 AB
                               36.8 AB
                                    11.1 A
                                         23.6 AB
24-4  8.3 A
          24.9 ABCD
                NT    0 A 18.7 AB
                               NT   NT   NT
25-6 10.4 AB
          33.3 ABCD
                 1.0 A
                     6.25 A
                          14.5 A
                               25.7 AB
                                    20.8 B
                                         NT
30-1 10.4 AB
          12.5 AB
                 7.3 AB
                     14.6 A
                          27.0 AB
                               29.9 AB
                                    18.0 AB
                                         13.2 B
23-5 18.7 AB
          33.3 ABCD
                12.5 B
                      2.1 A
                          35.4 AB
                               25.0 AB
                                    11.8 AB
                                         NT
70-1  4.2 A
          16.6 ABC
                 1.0 A
                      4.2 A
                          37.5 AB
                               16.7 B
                                    11.8 AB
                                         16.7 B
48-1 33.3 AB
          27.1 ABCD
                NT   NT   NT   NT   NT   NT
B-6  27.1 AB
          43.6 BCD
                NT   NT   NT   NT   NT   NT
C-3  22.9 AB
          43.7 BCD
                NT   NT   NT   NT   NT   NT
1986-41
      8.3 A
          22.9 ABCD
                 5.2 AB
                     NT   NT   NT   NT   NT
__________________________________________________________________________
 Values followed by the same letter are not significantly different
 according to Duncan's multiple range test (p = 0.05).
 NT = isolate not evaluated during this planting season.
Isolate 70-1 from Florida showed the highest efficacy of all isolates tested. This isolate has provided levels of protection identical to fungicide treatments and allowed for significantly higher stand counts than observed in the untreated controls in seven of the eight trials. Isolates 25-6 and 30-1 (both from the Southwest USA) have also been highly efficacious. Variation in efficacy for isolate 25-6 correlated with seasonal effects, having significantly improved stand count in only 33% of the trials conducted in the fall compared to 75% in the spring. While Rhizoctonia solani was occasionally recovered from diseased seedlings, this was at a low level, and the predominant cause of damping-off were phytopathogenic Pythium spp.
In addition to variation in efficacy as a biocontrol agent, there also is a high degree of variation in cultural characteristics among isolates of P. oligandrum. Differences in linear growth rates and temperature optima are often observed, as is production of zoosporangia and discharge of zoospores (Table 1). Variation among isolates is also observed with differences in oospore production, levels of spontaneous abortion, and germination frequency. Comparisons between isolates that were efficacious and nonefficacious in the field revealed that there is no correlation between efficacy and the particular cultural characteristics examined.
EXAMPLE 3
Root Colonization
When aseptically germinated tomato seed were colonized by P. oligandrum, in vitro, the mycelium was found primarily on the surface of the roots with no apparent visual symptoms of infection (e.g., necrosis or distortion of root morphology). When examined under the microscope, the fungus was found to occasionally penetrate an epidermal cell, but the hyphal growth was irregular in appearance and restricted to the single cell. Cell to cell growth was not observed. Therefore, under aseptic conditions, the subject biocontrol agent is primarily a surface colonizer of the root. When the seedlings were removed from the agar medium and washed prior to plating on fresh culture medium, low rates of recovery of P. oligandrum were observed, even though the fungus was observed microscopically on the root. This low frequency of recoverability may be one reason for not getting higher levels of root colonization from field grown plants as described below.
Recovery of P. oligandrum from roots of seedlings transplanted into the field was assessed by recovery of the seedlings from the field and gently removing adhering soil in water and plating on a medium that allows for identification of the biocontrol agent based on morphology. Low levels of root colonization by the biocontrol agent were observed.
In one trial, isolate 70-1 significantly reduced tomato damping-off, yet P. oligandrum was recovered at a frequency of only 0.1 colonies/cm of root. Even at the time of planting the frequency of recovery on selective medium was not high and was observed primarily on the tap root and crown regions of the seedling.
EXAMPLE 4
Formulations
Several different formulations have been evaluated for efficacy. A variety of different techniques can be used for production and formulation of biocontrol agents. Liquid cultures have been produced on a range of culture media containing readily available substrates such as homogenized vegetable juice. For example, in a preferred embodiment, production of oospores for conducting biocontrol trials can be done by growing cultures in a modified clarified V-8 juice broth culture (Ayers and Lumsden, 1975, Phytopathology 65:1094-1100). The medium is prepared by dissolving 1.5 g calcium carbonate in 200 ml of Cambells V-8 juice and pelleting the particulate matter by centrifugation. The supernatant is diluted with deionized water at a rate of 88 ml/l water and amended with cholesterol to a final concentration of 5 ppm. The medium is autoclaved prior to use.
Mycelial mats of the cultures are recovered on a sieve after 14 days growth at 25 C., rinsed in sterile water to remove medium and homogenized in a sterile blender. Mature thick walled oospores are counted with a hemacytometer and densities adjusted to desired levels prior to application to transplants. These have been formulated for application either directly to seeds or soil, mixed with a variety of materials for adhesion to seed surfaces, or encapsulated in sodium alginate. Liquid formulations have also been dried for addition to the soil either directly, mixed with kaolin dust, or coated onto perlite. Solid substrate fermentation using a variety of crop seeds also has been evaluated, U.S. Pat. No. 4,259,317.
1. Preferred Formulations
The preferred liquid preparation has been grown in several different media made from industrial byproducts or inexpensive, readily available components. Preferred dry formulations are either liquid fermentation biomass encapsulated in sodium alginate or pulverized dry fermentation products. Preliminary investigations on storage and survivability of inoculum have been conducted; with the dry formulation currently in use, a high level of survival is observed following eight weeks storage at room temperature.
2. Other Formulations
A. Wettable Powders
Wettable powders are water-dispersable compositions containing the active material, an inert solid extender, and one or more surfactants to provide rapid wetting and to prevent heavy flocculations when suspended in water.
The inert extenders which are preferred for use in the wettable powders of this invention containing the active compounds are of mineral or organic origin.
Extenders suitable for the wettable powder formulations of this invention are the natural clays, vermiculite, diatomaceous earth, and synthetic mineral fillers derived from silica and silicate. Most preferred filters for this invention are kaolinites, attapulgite clay, montmorillonite clays, synthetic silicas, synthetic magnesium silicate, and calcium sulfate dihydrate. A surface active agent can also be added to give a homogenous and stable formulation.
Among the more preferred surfactants are the nonionic and anionic types. They are most suitable for the preparation of dry, wettable products of this invention and dispersants. Occasionally a liquid, non-ionic compound which is primarily an emulsifier may serve as both wetter and dispersant.
Most preferred wetting agents are alkylbenzene and alkylnaphthalene sulfonates, sulfated fatty alcohols, amines, or acid amides, long chain esters of sodium isethionate, esters of sodium sulfosuccinate, sulfated or sulfonated vegetable oils, and ditertiary acetylenic glycols. Preferred dispersants are methyl cellulose, polyvinyl alcohol, lignin sulfonates, polymeric alkylnaphthalene sulfonates, sodium naphthalene sulfonates, polymethylene bisnaphthalene sulfonate, and sodium-N-methyl-N-(long chain acid) taruates.
Wetting and dispersing agents in these preferred wettable powder compositions of the invention are usually present at concentrations of from about 0.5 weight percent to 5 weight percent. The inert extender then completes the formulation. Where needed, 0.1 weight percent of the extender may be replaced by a corrosion inhibitor or an anti-foaming agent or both.
Thus, wettable powder contains a corrosion inhibitor or an anti-foaming agent or both, the corrosion inhibitor should not exceed about 1 percent of the composition, and the anti-foaming agent should not exceed about 0.5 percent by weight of the composition, both replacing equivalent amounts of the inert extender.
B. Dusts
Dusts are dense powder compositions which are intended for application in dry form. Dusts are characterized by their free-flowing and rapid settling properties so that they are not readily windborne to areas where their presence is not desired. They contain primarily an active ingredient and a dense, free-flowing, solid extender. Their performance is sometimes aided by the inclusion of a wetting agent and convenience in manufacture frequently demands the inclusion of an inert absorptive grinding aid.
The wettable powder as described above can also be used in the preparation of dusts. While such wettable powders can be used directly in dust form, it is more advantageous to dilute them by blending with the dense dust diluent. In this manner, dispersing agents, corrosion inhibitors, and anti-foam agents may also be used as components of a dust.
Thus, the dust compositions of this invention can comprise from about 0.5 to 20.0 weight percent active ingredient, 5 to 25 weight percent filler, 0.0 to 1.0 weight percent wetting agent, and from about 30 to 90 weight percent dense, free-flowing extender, as these terms are used herein. Such dust formulations can contain, in addition, minor amounts of dispersants, corrosion inhibitors, and anti-foam agents derived from the wettable powders used to make the dust.
C. Emulsifiable Oils
Emulsifiable oils are usually solutions or suspensions of active material in non-water miscible solvents together with a surfactant and/or emulsifier.
For compositions of this invention, emulsifiable oil compositions can be made by mixing the active ingredient with an organic solvent and surfactant. Suitable solvents for the compositions of this invention are chlorinated solvents, water immiscible ethers, esters, or ketones alone or in admixture with aromatic hydrocarbons. Suitable surfactants are those ionic or non-ionic agents known to the art as emulsifying agents.
Emulsifying agents most suitable for the emulsifiable oil compositions of this invention are long chain alkyl or mercaptan polyethoxy alcohols, alkylaryl polyethoxy alcohols, sorbitan fatty acid esters, polyoxyethylene ethers with sorbitan fatty acid esters, polyethylene glycol esters with fatty rosin acids, fatty alkylol amide condensates, calcium and amine salts of fatty alcohol sulfates, oil soluble petroleum sulfonates, or preferably mixtures of these emulsifying agents should comprise from about 1 to 10 weight percent of the total composition. As described above, however, up to 5 parts of emulsifying agent for each part of active ingredient can be used.
Thus, emulsifiable oil compositions of the present invention can consist of from about 10 to 50 weight percent active ingredient, about 40 to 82 percent solvents, and about 1 to 10 weight percent emulsifier, as these terms are defined and used above.
D. Granules
Granules are physically stable, particulate compositions containing spores and/or mycelia of this invention which adhere to or are distributed through a basic matrix of a coherent, inert carrier with microscopic dimensions. In order to aid leaching of the active ingredient from the granule, a surfactant can be present.
The inert carrier is preferably of mineral origin, and suitable carriers are natural clays, some pyrophyllites and vermiculite. Suitable wetting agents can be anionic or non-ionic.
For the granule compositions of this invention, most suitable carriers are to two types. The first are porous, absorptive pre-formed granules, such as preformed and screened granular attapulgite or heat expanded, granular, screened vermiculite. On either of these, a solution of the active agent can be sprayed and will be absorbed at concentrations up to 25 weight percent of the total weight. The second type are initially powdered kaolin clays, hydrated attapulgite, or bentonite clays in the form of sodium calcium, or magnesium bentonites. Water-soluble salts such as sodium salts may also be present to aid in the disintegrations of the granules in the presence of moisture. These ingredients are blended with the active component distributed uniformly throughout the mass. Such granules can also be made with 25 to 30 weight percent active component but more frequently a concentration of about 10 weight percent is desired for optimum distribution. The granular compositions of this invention are believed to be most useful in a size range of 15-30 mesh.
The most suitable wetting agents for the granular compositions of this invention depend upon the type of granule used. When pre-formed granules are sprayed with active material in liquid form, the most suitable wetting agents are non-ionic, liquid wetters miscible with the solvent. These are more generally known in the art as emulsifiers and comprise alkylaryl polyether alcohols, alkyl polyether alcohols, polyoxethylene sorbitan fatty acid esters, polyethylene glycol esters with fatty or rosin acids, fatty alkylol amide condensates, oil petroleum or vegetable oil sulfonates, or mixtures of these. Such agents will usually comprise up to about 5 weight percent of the total composition.
When the active ingredient is first mixed with a powdered carrier and subsequently granulated, liquid non-ionic wetters can still be used, but it is usually preferable to incorporate at the mixing stage one of the solid, powdered anionic wetting agents such as those previously listed for the wettable powders. Such agents should comprise about 0 to 2 percent of the total composition.
Thus, the preferred granular formulation of this invention comprises about 5 to 30 weight percent active material, about 0 to 5 weight percent wetting agent, and about 65 to 95 percent inert mineral carrier, as these terms are used herein.
EXAMPLE 5
Seed Coating Evaluations
The survivability of oospores from isolates efficacious in transplant trials when coated on the surface of tomato, cucumber, and soybean seeds was evaluated. Different types of adhering materials (carboxymethyl cellulose, sodium alginate, pelgel, nitracoat, and others) have been evaluated in these trials. Depending on the treatment that the biocontrol preparation received, significant levels of oospore survival were observed following 16 weeks storage at room temperature.
EXAMPLE 6
Molecular Identification of Pythium oligandrum
With more than 120 species in the genus Pythium, accurate identification of isolates can be difficult, particularly for species that share many morphological similarities. Therefore, unambiguous identification of isolates is preferred. The mitochondrial DNA (mtDNA) is an advantageous molecular marker for use with isolates of genus Pythium. The Pythium mtDNA is highly conserved within a species yet divergent between species to allow differentiation by RFLP analysis of even morphologically similar species. Detailed restriction maps have been constructed for 18 species in the genus and numerous geographically separated isolates of each species to evaluate both inter- as well as intra-specific variation of the genome. This research has supported the validity of using the mitochondrial DNA for taxonomic classification of species in the genus. By examining the mtDNA RFLPs and restriction maps, the isolates used as biocontrol agents described herein have been unequivocally identified as the nonphytopathogenic species P. oligandrum. The mitochondrial genome also has proved to be useful for construction of species, and in some cases isolate specific molecular markers. The organization of the mitochondrial genome in Pythium is unusual in that approximately 80% of the genome is comprised of an inverted repeat. The inverted repeats are separated by two single copy unique regions referred to as the small and large unique region (which is indicative of their relative sizes). It is predominantly in the small unique region where intraspecific variation in restriction maps for this species is observed (Genome 34:156-162). While not included in the previously cited reference, isolate 70-1 has a mtDNA restriction map similar to isolate 82-24. The use of sequences from the small unique region are useful for constructing probes with varying levels of species and isolate specificity (Phytopathology 81:742-746). Subsequent DNA sequence analysis has identified regions of sequence variation which should enhance the prospects for constructing isolate specific probes or PCR primers (See SEQ ID. NOs. 1-8).
EXAMPLE 7
Regions of DNA Sequence Variation Among Isolates of Pythium oligandrum
The small unique single copy region of the mitochondrial genome and adjacent inverted repeat (IR) regions were cloned and sequenced for several isolates of P. oligandrum (shown as SEQ ID NOs. 1-8). Sequence variation in these regions was found among all isolates except two (1985-5 SEQ ID NO. 2! and 1986-41 SEQ ID NO. 3!), providing a means for differentiating most isolates. A general outline of where these sequence variations were found follows.
Inverted Repeat
Among all isolates examined, sequence comparisons in the IR region are conserved with the following exceptions (data presented for only one arm of the inverted repeat):
1982-24 (SEQ ID NO. 1), 1986-41 (SEQ ID. NO. 3), 1985-5 (SEQ ID NO. 2), 17-1 (SEQ ID NO. 4), and 1986-43 (SEQ ID NO. 6) have an extra "A" at base 307.
1986-42 (SEQ ID NO. 6), 27-6 (SEQ ID NO. 7), and 30-1 (SEQ ID NO. 8) have an extra "A" at base 451.
1986-42 (SEQ ID NO. 6) has a deletion of 285 bp relative to isolate 17-1 (SEQ ID NO. 4) that removes a portion of the small unique and IR region, causing the IR region to be smaller than 17-1 by 234 bp. This deletion also is observed when comparing 1986-42 (SEQ ID NO. 6) to all other isolates, although the size of the deletion varies.
1982-24 (SEQ ID NO. 1), 1985-5 (SEQ ID NO. 2), and 1986-41 (SEQ ID NO. 3) have inverted repeats that are longer than the other isolates examined by approximately 774 bp (exact number varies depending on the isolate).
1986-41 (SEQ ID NO. 3) has an extra "AATA" in the IR relative to 1982-24 (SEQ ID NO. 1) and 1985-5 (SEQ ID NO. 2) starting at base 696.
Single Copy Small Unique Region
This region contains sequences that are most effective in exhibiting sequence uniqueness (except for 1985-5 SEQ ID NO. 2! and 1986-41 SEQ ID NO. 3!, which are the same). The relative position of this region for each isolate is shown in Table 3.
              TABLE 3
______________________________________
Positions of unique regions in isolates
Isolate
       SEQ ID NO.
                 position of unique region (base #s)
______________________________________
1982-24
       1         1278-2649
1985-5 2         1281-2653
1986-41
       3         1281-2653
17-1   4         504-715
23-5   5         502-684
1986-42
       6         270-664
27-6   7         504-?
                 (region only partially sequenced to base 565)
30-1   8         504-?
                 (region only partially sequenced to base
______________________________________
                 612)
Some specific regions of sequence variation are shown in Table 4.
              TABLE 4
______________________________________
SEQ ID NOs. Regions of variation
______________________________________
2 vs. 1     base 1914 and 1910, respectively
3 vs. 1     base 1914 and 1910, respectively
4 vs. 8     base 562, 585, 608
4 (8) vs. 6 bases 698-954 of SEQ ID NO. 4 deleted in
            SEQ ID NO. 6
            bases 500-550 of SEQ ID NO. 4 deleted in
            SEQ ID NO. 6
4 (8) vs. 5 bases 500-550 of SEQ ID NO. 4 deleted in
            SEQ ID NO. 5
4 (8) vs. 7 bases 500-550 of SEQ ID NO. 4 deleted in
            SEQ ID NO. 7
5 vs.       base 451, SEQ ID NO. 7 has an extra "A"
            base 510 and 511, respectively
            base 515 and 516, respectively
            base 555 and 556, respectively
______________________________________
EXAMPLE 8
Evaluation of Plant Pathogenicity
In his initial description of the species, Drechsler (1946) indicated the P. oligandrum could be isolated from necrotic tissue, but when tested for pathogenicity it did not infect plants. His conclusion was that this species was able to colonize tissue after it had been colonized by a pathogen. When coated on seed surfaces, P. oligandrum was found to be nonpathogenic in vitro and in vivo on 12 crop species representing six families (Martin and Hancock, 1987). When planted in fumigated soil, there was no reduction in shoot weight of stand counts. In addition, reduction of root densities was not observed when the plants were grown in field soil. Evaluations of pathogenicity also were conducted with several ornamental crops; none was observed. Pythium oligandrum also has been reported to be nonpathogenic on barley and oats (Kilpatrick, 1968, Plant Dis. Rep. 52:209-212; Bratoloveanu and Wallace, 1982, Biennial Report of the Waite Agricultural Research Institute 85:143 South Australia), pineapple (Klemmer and Nakano, 1964, Plant Dis. Rep. 48:848-852), cress (Al-Hamdani, 1982, Ph.D. dissertation, Dept. of Botany, University of Sheffield; Al-Hamdani et al., 1983, Plant Pathology 32:449-454; Lutchmeah and Cooke, 1984, Trans. Brit. Mycol. Soc. 83:696-700), carrot (Lutchmeah and Cooke, 1984), sugarbeet (O'Sullivan and Kavanagh, 1992, Plant Pathology 41:582-590), and several ornamental crops (Kelling, 1985, Nachrichtenblatt fur den Pflanzenschutz in der DDR 39:191-193). The colonization of tomato seedlings in vitro by P. oligandrum has been examined microscopically. Fungal hyphae grew over the surface of the root and occasionally penetrated a single cell in the top layer of the epidermis. However, hyphal growth within the plant cell was restricted with a knobby-like appearance and did not grow into adjacent cells.
It should be understood that the examples and embodiments described herein are for illustrative purposes only and that various modifications or changes in light thereof will be suggested to persons skilled in the art and are to be included within the spirit and purview of this application and the scope of the appended claims.
__________________________________________________________________________
#             SEQUENCE LISTING
- (1) GENERAL INFORMATION:
-    (iii) NUMBER OF SEQUENCES: 8
- (2) INFORMATION FOR SEQ ID NO:1:
-      (i) SEQUENCE CHARACTERISTICS:
#pairs    (A) LENGTH: 3926 base
          (B) TYPE: nucleic acid
          (C) STRANDEDNESS: single
          (D) TOPOLOGY: linear
-     (ii) MOLECULE TYPE: DNA (genomic)
-     (vi) ORIGINAL SOURCE:
#1982-24  (C) INDIVIDUAL ISOLATE:
-     (xi) SEQUENCE DESCRIPTION: SEQ ID NO:1:
- CTGCAGCTGA ATCTGCTATA GGTTTAGCAA TAATGATTGT TTTTTTCAAA AT - #ATATGGAG
  60
- ATATATCTAT TTATAAAATT AATCTATTAT CTTTATAGAT TAATTTTATA AG - #TATACATA
 120
- TAATTAATAA TATTTCTATT TCGTATTGAA ATAAAAATAT TTTTTATTAA CT - #TAAATTAA
 180
- AAAGCGAATA AAATTAAGAA AGCAATCATT AAACAGAATA AAGCAATAGA TT - #CAGTTAAA
 240
- GCGAAACCTA AAATAGCTGT TCTTGTTAAA TCTTGTTGTA AAGAAGGGTT TC - #TAGAAATA
 300
- CCTAAAACTA ATGAACTAAA TACTGAACCG ATACCGATAC CAGCACCTGC TA - #ATCCAATA
 360
- GTAGCTAATC CAGCACCAAT AAATTTTGCA GATTGTAATA ACATATTATG TA - #ATTAATTT
 420
- ATATCTTTTT AAAGATATAT AACTTTTAAA AAAAAATTAA AATGAAAATA CT - #TCTAATAA
 480
- GAATATATTT TATTATAAAT ATTAATTATT TATTTCTTAT TAAAATATTA TG - #ATTATTTA
 540
- TTAAAGTAGA ATAAGGATTA CAATTTTCTG TTAAAAAAAT AAAACCTTTC TC - #TATTGAAG
 600
- AATTTTTTAT AGCTACTGTT TAATTAAAAA AGTTTATAAT TTAATTCTTT TA - #TAGAACAT
 660
- TTAAAAAAAA ATATTATTAA TGGTAGAATT GAGAGAAATA CTTCTAATTT AC - #TTTATATT
 720
- AATAATATAG GAAATAATGA TATGATTGAT ACAAATACAA TTATTGAATT AA - #ATAATTCA
 780
- ACTACTTCCG AAAGAAGAAT GGAATTTATG AATAGTATTA TACATCACGA AA - #ATAATAAT
 840
- GAAAATCGTG CTCTATTAAT TGAACATAGT TCACCAGAAG TAAGGACTTA TT - #TACACGAG
 900
- TTATTAATTA GATCAGCAAA TAATTCAAAT ATAACTGAAG AGGTTTTATA TA - #GAATAGGA
 960
- AACATTTTCC TTTATACAAT ATCCAATTTA GATATAGACG GATTAGTTCT TA - #GAGATGTG
1020
- ATTCAAAATA TGAGAGAATC TATGGTTATG TTTAACACAA ATCAAATTTA CT - #CTATACTT
1080
- GAAAATCAAG TTAGTAACCA TAATCAATAT TTAGAAGAGA TTAGGTTAGC GA - #GTGAGGAA
1140
- CATATTGATG AGCGCGTTCA AGAATTTCAT CGAGAAGTAG ATCAGAAAAT AG - #CTTTAAAT
1200
- CGAAATGGAA TATTAGGATC AATGGCTTTA ACTTCTATAG GAGTTCCTCA AA - #TTGTGAGT
1260
- GGATTAGTAG CAAGATCGGT TTTATTTTGA AACTCTATCG AGTTTATTTT CT - #TTGAATTT
1320
- TTCTAATATT TTATCCTCTA TTTTGTTATC GTTTTTGTCT ACTTTATATA TT - #AATAAAAT
1380
- TTTTTTTCCT AATATTTCAA ATTTTGATTT ATTTTTGTAT ATATTTTCTT AA - #ATTTTCTA
1440
- ACTCTTTAGC ATCTTCTATT TGAAAAAAAT CAATTAATAA ACTAGCTTCA TC - #TCTTGTTA
1500
- ACCCGTGAGT AGTTAGTGTT GTAAAAGGAC AAGCTGCTAC ATCTGACTGT GA - #GTTTATTC
1560
- TCCAAAATTT AGCAATTAAT TTTTCTTCTT CATTTAAAAC GATTTCTGGT GA - #ATTAAAAA
1620
- ATTTCTCAAT AAGTTGTGTT ATCTCCAACG GTATTTCGTT TTCATTTAAA CA - #CACATCAT
1680
- TGAATATATA TATATTAAAA ATTAAGATTA ATATAAATAT TGTAATATTT TT - #ATTTTTGA
1740
- TTTCCATAAT TAATTGTTTT TATAATTAAA TTAGGTAAAG TAGTATCGAC GC - #CTAGTAGT
1800
- CCTAAACATA TTATACCTCC ACCTATTAAT ATTTTCTTTT TCAATTTTTT AG - #CGTGTTCT
1860
- TCACGTTCTT TTTGAAAAGT TTCTGCTCTC TCCTCTATTC CTTGAATAAA AT - #TATTTGTA
1920
- ATTTCTTCTA GTTCTTGAGA ATTTTTGAGC TTTATTTCTT CTAAATATTT AT - #TAAAAGTA
1980
- GTTATTTGTT TATCTAAATC GATTGATATT TGATTTATGT TATAAATACA CA - #TTGTTTCA
2040
- CTTATCTTCT TCATAAAATC TCTTACTAAT AATCCCTCTA TTTCTAAATT CG - #ATATCGTA
2100
- TAAAGAAAAA TGTTTCCTAT TCGATAGAAA TCTTCTTCAG TTATATTTGA AT - #TAATTGCT
2160
- GTTCTTCTTA ATAAATCATT TATATAAGTT CTCACGTGAG GTGAGCTATT TT - #CTATTAAT
2220
- GATAAAAGAT TTTCACTATT ATTTTCGTGA TTTATAATAC TATTCATAAT CT - #CTAATCTT
2280
- CTTTCAGAAG ATATGTGGTT ATTTAATTCA ATAATTGTTT GAGAATCAAT TG - #ATTCTATA
2340
- CCATTTAACT TTTTTATATA TGGTAATTTA TCTATATTAT TTAAAAGATG AT - #GATTTATC
2400
- TTATCTCTAA AACTTTCCTG TAAATTAAAA TTAGGAGGTT TTATTGGTGA AC - #CTTTTTCT
2460
- TCAAATAATA AGTTGCCTAA TTTTAAGAAA TCTTCTGATT TAAAGTCTAT AT - #TATTGTTT
2520
- ATCATATTTT ATTTATTAAA AGACTTAAGA GTATTATAAA ATAATTTAAT AC - #CTTCATCT
2580
- AAAATATCCC TGAAACGGAT AATTCCTTCA GCCTCTGTTA ATTGAACTGT TG - #TAACAGGG
2640
- GATATTACTG ATCTTGCTAC TAATCCACTC ACAATTTGAG GAACTCCTAT AG - #AAGTTAAA
2700
- GCCATTGATC CTAATATTCC ATTTCGATTT AAAGCTATTT TCTGATCTAC TT - #CTCGATGA
2760
- AATTCTTGAA CGCGCTCATC AATATGTTCC TCACTCGCTA ACCTAATCTC TT - #CTAAATAT
2820
- TGATTATGGT TACTAACTTG ATTTTCAAGT ATAGAGTAAA TTTGATTTGT GT - #TAAACATA
2880
- ACCATAGATT CTCTCATATT TTGAATCACA TCTCTAAGAA CTAATCCGTC TA - #TATCTAAA
2940
- TTGGATATTG TATAAAGGAA AATGTTTCCT ATTCTATATA AAACCTCTTC AG - #TTATATTT
3000
- GAATTATTTG CTGATCTAAT TAATAACTCG TGTAAATAAG TCCTTACTTC TG - #GTGAACTA
3060
- TGTTCAATTA ATAGAGCACG ATTTTCATTA TTATTTTCGT GATGTATAAT AC - #TATTCATA
3120
- AATTCCATTC TTCTTTCGGA AGTAGTTGAA TTATTTAATT CAATAATTGT AT - #TTGTATCA
3180
- ATCATATCAT TATTTCCTAT ATTATTAATA TAAAGTAAAT TAGAAGTATT TC - #TCTCAATT
3240
- CTACCATTAA TAATATTTTT TTTTAAATGT TCTATAAAAG AATTAAATTA TA - #AACTTTTT
3300
- TAATTAAACA GTAGCTATAA AAAATTCTTC AATAGAGAAA GGTTTTATTT TT - #TTAACAGA
3360
- AAATTGTAAT CCTTATTCTA CTTTAATAAA TAATCATAAT ATTTTAATAA GA - #AATAAATA
3420
- ATTAATATTT ATAATAAAAT ATATTCTTAT TAGAAGTATT TTCATTTTAA TT - #TTTTTTTA
3480
- AAAGTTATAT ATCTTTAAAA AGATATAAAT TAATTACATA ATATGTTATT AC - #AATCTGCA
3540
- AAATTTATTG GTGCTGGATT AGCTACTATT GGATTAGCAG GTGCTGGTAT CG - #GTATCGGT
3600
- TCAGTATTTA GTTCATTAGT TTTAGGTATT TCTAGAAACC CTTCTTTACA AC - #AAGATTTA
3660
- ACAAGAACAG CTATTTTAGG TTTCGCTTTA ACTGAATCTA TTGCTTTATT CT - #GTTTAATG
3720
- ATTGCTTTCT TAATTTTATT CGCTTTTTAA TTTAAGTTAA TAAAAAATAT TT - #TTATTTCA
3780
- ATACGAAATA GAAATATTAT TAATTATATG TATACTTATA AAATTAATCT AT - #AAAGATAA
3840
- TAGATTAATT TTATAAATAG ATATATCTCC ATATATTTTG AAAAAAACAA TC - #ATTATTGC
3900
#            3926  TCAG CTGCAG
- (2) INFORMATION FOR SEQ ID NO:2:
-      (i) SEQUENCE CHARACTERISTICS:
#pairs    (A) LENGTH: 3926 base
          (B) TYPE: nucleic acid
          (C) STRANDEDNESS: single
          (D) TOPOLOGY: linear
-     (ii) MOLECULE TYPE: DNA (genomic)
-     (vi) ORIGINAL SOURCE:
          (B) STRAIN: 1985-5
-     (xi) SEQUENCE DESCRIPTION: SEQ ID NO:2:
- CTGCAGCTGA ATCTGCTATA GGTTTAGCAA TAATGATTGT TTTTTTCAAA AT - #ATATGGAG
  60
- ATATATCTAT TTATAAAATT AATCTATTAT CTTTATAGAT TAATTTTATA AG - #TATACATA
 120
- TAATTAATAA TATTTCTATT TCGTATTGAA ATAAAAATAT TTTTTATTAA CT - #TAAATTAA
 180
- AAAGCGAATA AAATTAAGAA AGCAATCATT AAACAGAATA AAGCAATAGA TT - #CAGTTAAA
 240
- GCGAAACCTA AAATAGCTGT TCTTGTTAAA TCTTGTTGTA AAGAAGGGTT TC - #TAGAAATA
 300
- CCTAAAACTA ATGAACTAAA TACTGAACCG ATACCGATAC CAGCACCTGC TA - #ATCCAATA
 360
- GTAGCTAATC CAGCACCAAT AAATTTTGCA GATTGTAATA ACATATTATG TA - #ATTAATTT
 420
- ATATCTTTTT AAAGATATAT AACTTTTAAA AAAAAATTAA AATGAAAATA CT - #TCTAATAA
 480
- GAATATATTT TATTATAAAT ATTAATTATT TATTTCTTAT TAAAATATTA TG - #ATTATTTA
 540
- TTAAAGTAGA ATAAGGATTA CAATTTTCTG TTAAAAAAAT AAAACCTTTC TC - #TATTGAAG
 600
- AATTTTTTAT AGCTACTGTT TAATTAAAAA AGTTTATAAT TTAATTCTTT TA - #TAGAACAT
 660
- TTAAAAAAAA ATATTATTAA TGGTAGAATT GAGAGAAATA CTTCTAATTT AC - #TTTATATT
 720
- AATAATATAG GAAATAATGA TATGATTGAT ACAAATACAA TTATTGAATT AA - #ATAATTCA
 780
- ACTACTTCCG AAAGAAGAAT GGAATTTATG AATAGTATTA TACATCACGA AA - #ATAATAAT
 840
- GAAAATCGTG CTCTATTAAT TGAACATAGT TCACCAGAAG TAAGGACTTA TT - #TACACGAG
 900
- TTATTAATTA GATCAGCAAA TAATTCAAAT ATAACTGAAG AGGTTTTATA TA - #GAATAGGA
 960
- AACATTTTCC TTTATACAAT ATCCAATTTA GATATAGACG GATTAGTTCT TA - #GAGATGTG
1020
- ATTCAAAATA TGAGAGAATC TATGGTTATG TTTAACACAA ATCAAATTTA CT - #CTATACTT
1080
- GAAAATCAAG TTAGTAACCA TAATCAATAT TTAGAAGAGA TTAGGTTAGC GA - #GTGAGGAA
1140
- CATATTGATG AGCGCGTTCA AGAATTTCAT CGAGAAGTAG ATCAGAAAAT AG - #CTTTAAAT
1200
- CGAAATGGAA TATTAGGATC AATGGCTTTA ACTTCTATAG GAGTTCCTCA AA - #TTGTGAGT
1260
- GGATTAGTAG CAAGATCGGT TTTATTTTGA AACTCTATCG AGTTTATTTT CT - #TTGAATTT
1320
- TTCTAATATT TTATCCTCTA TTTTGTTATC GTTTTTGTCT ACTTTATATA TT - #AATAAAAT
1380
- TTTTTTTCCT AATATTTCAA ATTTTGATTT ATTTTTGTAT ATATTTTCTT AA - #ATTTTCTA
1440
- ACTCTTTAGC ATCTTCTATT TGAAAAAAAT CAATTAATAA ACTAGCTTCA TC - #TCTTGTTA
1500
- ACCCGTGAGT AGTTAGTGTT GTAAAAGGAC AAGCTGCTAC ATCTGACTGT GA - #GTTTATTC
1560
- TCCAAAATTT AGCAATTAAT TTTTCTTCTT CATTTAAAAC GATTTCTGGT GA - #ATTAAAAA
1620
- ATTTCTCAAT AAGTTGTGTT ATCTCCAACG GTATTTCGTT TTCATTTAAA CA - #CACATCAT
1680
- TGAATATATA TATATTAAAA ATTAAGATTA ATATAAATAT TGTAATATTT TT - #ATTTTTGA
1740
- TTTCCATAAT TAATTGTTTT TATAATTAAA TTAGGTAAAG TAGTATCGAC GC - #CTAGTAGT
1800
- CCTAAACATA TTATACCTCC ACCTATTAAT ATTTTCTTTT TCAATTTTTT AG - #CGTGTTCT
1860
- TCACGTTCTT TTTGAAAAGT TTCTGCTCTC TCCTCTATTC CTTGAATAAA AT - #TATTTGTA
1920
- ATTTCTTCTA GTTCTTGAGA ATTTTTGAGC TTTATTTCTT CTAAATATTT AT - #TAAAAGTA
1980
- GTTATTTGTT TATCTAAATC GATTGATATT TGATTTATGT TATAAATACA CA - #TTGTTTCA
2040
- CTTATCTTCT TCATAAAATC TCTTACTAAT AATCCCTCTA TTTCTAAATT CG - #ATATCGTA
2100
- TAAAGAAAAA TGTTTCCTAT TCGATAGAAA TCTTCTTCAG TTATATTTGA AT - #TAATTGCT
2160
- GTTCTTCTTA ATAAATCATT TATATAAGTT CTCACGTGAG GTGAGCTATT TT - #CTATTAAT
2220
- GATAAAAGAT TTTCACTATT ATTTTCGTGA TTTATAATAC TATTCATAAT CT - #CTAATCTT
2280
- CTTTCAGAAG ATATGTGGTT ATTTAATTCA ATAATTGTTT GAGAATCAAT TG - #ATTCTATA
2340
- CCATTTAACT TTTTTATATA TGGTAATTTA TCTATATTAT TTAAAAGATG AT - #GATTTATC
2400
- TTATCTCTAA AACTTTCCTG TAAATTAAAA TTAGGAGGTT TTATTGGTGA AC - #CTTTTTCT
2460
- TCAAATAATA AGTTGCCTAA TTTTAAGAAA TCTTCTGATT TAAAGTCTAT AT - #TATTGTTT
2520
- ATCATATTTT ATTTATTAAA AGACTTAAGA GTATTATAAA ATAATTTAAT AC - #CTTCATCT
2580
- AAAATATCCC TGAAACGGAT AATTCCTTCA GCCTCTGTTA ATTGAACTGT TG - #TAACAGGG
2640
- GATATTACTG ATCTTGCTAC TAATCCACTC ACAATTTGAG GAACTCCTAT AG - #AAGTTAAA
2700
- GCCATTGATC CTAATATTCC ATTTCGATTT AAAGCTATTT TCTGATCTAC TT - #CTCGATGA
2760
- AATTCTTGAA CGCGCTCATC AATATGTTCC TCACTCGCTA ACCTAATCTC TT - #CTAAATAT
2820
- TGATTATGGT TACTAACTTG ATTTTCAAGT ATAGAGTAAA TTTGATTTGT GT - #TAAACATA
2880
- ACCATAGATT CTCTCATATT TTGAATCACA TCTCTAAGAA CTAATCCGTC TA - #TATCTAAA
2940
- TTGGATATTG TATAAAGGAA AATGTTTCCT ATTCTATATA AAACCTCTTC AG - #TTATATTT
3000
- GAATTATTTG CTGATCTAAT TAATAACTCG TGTAAATAAG TCCTTACTTC TG - #GTGAACTA
3060
- TGTTCAATTA ATAGAGCACG ATTTTCATTA TTATTTTCGT GATGTATAAT AC - #TATTCATA
3120
- AATTCCATTC TTCTTTCGGA AGTAGTTGAA TTATTTAATT CAATAATTGT AT - #TTGTATCA
3180
- ATCATATCAT TATTTCCTAT ATTATTAATA TAAAGTAAAT TAGAAGTATT TC - #TCTCAATT
3240
- CTACCATTAA TAATATTTTT TTTTAAATGT TCTATAAAAG AATTAAATTA TA - #AACTTTTT
3300
- TAATTAAACA GTAGCTATAA AAAATTCTTC AATAGAGAAA GGTTTTATTT TT - #TTAACAGA
3360
- AAATTGTAAT CCTTATTCTA CTTTAATAAA TAATCATAAT ATTTTAATAA GA - #AATAAATA
3420
- ATTAATATTT ATAATAAAAT ATATTCTTAT TAGAAGTATT TTCATTTTAA TT - #TTTTTTTA
3480
- AAAGTTATAT ATCTTTAAAA AGATATAAAT TAATTACATA ATATGTTATT AC - #AATCTGCA
3540
- AAATTTATTG GTGCTGGATT AGCTACTATT GGATTAGCAG GTGCTGGTAT CG - #GTATCGGT
3600
- TCAGTATTTA GTTCATTAGT TTTAGGTATT TCTAGAAACC CTTCTTTACA AC - #AAGATTTA
3660
- ACAAGAACAG CTATTTTAGG TTTCGCTTTA ACTGAATCTA TTGCTTTATT CT - #GTTTAATG
3720
- ATTGCTTTCT TAATTTTATT CGCTTTTTAA TTTAAGTTAA TAAAAAATAT TT - #TTATTTCA
3780
- ATACGAAATA GAAATATTAT TAATTATATG TATACTTATA AAATTAATCT AT - #AAAGATAA
3840
- TAGATTAATT TTATAAATAG ATATATCTCC ATATATTTTG AAAAAAACAA TC - #ATTATTGC
3900
#            3926  TCAG CTGCAG
- (2) INFORMATION FOR SEQ ID NO:3:
-      (i) SEQUENCE CHARACTERISTICS:
#pairs    (A) LENGTH: 3933 base
          (B) TYPE: nucleic acid
          (C) STRANDEDNESS: single
          (D) TOPOLOGY: linear
-     (ii) MOLECULE TYPE: DNA (genomic)
-     (vi) ORIGINAL SOURCE:
#1986-41  (C) INDIVIDUAL ISOLATE:
-     (xi) SEQUENCE DESCRIPTION: SEQ ID NO:3:
- CTGCAGCTGA ATCTGCTATA GGTTTAGCAA TAATGATTGT TTTTTTCAAA AT - #ATATGGAG
  60
- ATATATCTAT TTATAAAATT AATCTATTAT CTTTATAGAT TAATTTTATA AG - #TATACATA
 120
- TAATTAATAA TATTTCTATT TCGTATTGAA ATAAAAATAT TTTTTATTAA CT - #TAAATTAA
 180
- AAAGCGAATA AAATTAAGAA AGCAATCATT AAACAGAATA AAGCAATAGA TT - #CAGTTAAA
 240
- GCGAAACCTA AAATAGCTGT TCTTGTTAAA TCTTGTTGTA AAGAAGGGTT TC - #TAGAAATA
 300
- CCTAAAACTA ATGAACTAAA TACTGAACCG ATACCGATAC CAGCACCTGC TA - #ATCCAATA
 360
- GTAGCTAATC CAGCACCAAT AAATTTTGCA GATTGTAATA ACATATTATG TA - #ATTAATTT
 420
- ATATCTTTTT AAAGATATAT AACTTTTAAA AAAAAATTAA AATGAAAATA CT - #TCTAATAA
 480
- GAATATATTT TATTATAAAT ATTAATTATT TATTTCTTAT TAAAATATTA TG - #ATTATTTA
 540
- TTAAAGTAGA ATAAGGATTA CAATTTTCTG TTAAAAAAAT AAAACCTTTC TC - #TATTGAAG
 600
- AATTTTTTAT AGCTACTGTT TAATTAAAAA AGTTTATAAT TTAATTCTTT TA - #TAGAACAT
 660
- TTAAAAAAAA ATATTATTAA TGGTAGAATT GAGAGAAATA AATACTTCTA AT - #TTACTTTA
 720
- TATTAATAAT ATAGGAAATA ATGATATGAT TGATACAAAT ACAATTATTG AA - #TTAAATAA
 780
- TTCAACTACT TCCGAAAGAA GAATGGAATT TATGAATAGT ATTATACATC AC - #GAAAATAA
 840
- TAATGAAAAT CGTGCTCTAT TAATTGAACA TAGTTCACCA GAAGTAAGGA CT - #TATTTACA
 900
- CGAGTTATTA ATTAGATCAG CAAATAATTC AAATATAACT GAAGAGGTTT TA - #TATAGAAT
 960
- AGGAAACATT TTCCTTTATA CAATATCCAA TTTAGATATA GACGGATTAG TT - #CTTAGAGA
1020
- TGTGATTCAA AATATGAGAG AATCTATGGT TATGTTTAAC ACAAATCAAA TT - #TACTCTAT
1080
- ACTTGAAAAT CAAGTTAGTA ACCATAATCA ATATTTAGAA GAGATTAGGT TA - #GCGAGTGA
1140
- GGAACATATT GATGAGCGCG TTCAAGAATT TCATCGAGAA GTAGATCAGA AA - #ATAGCTTT
1200
- AAATCGAAAT GGAATATTAG GATCAATGGC TTTAACTTCT ATAGGAGTTC CT - #CAAATTGT
1260
- GAGTGGATTA GTAGCAAGAT CGGTTTTATT TTGAAACTCT ATCGAGTTTA TT - #TTCTTTGA
1320
- ATTTTTCTAA TATTTTATCC TCTATTTTGT TATCGTTTTT GTCTACTTTA TA - #TATTAATA
1380
- AAATTTTTTT TCCTAATATT TCAAATTTTG ATTTATTTTT GTATATATTT TC - #TTAAATTT
1440
- TCTAACTCTT TAGCATCTTC TATTTGAAAA AAATCAATTA ATAAACTAGC TT - #CATCTCTT
1500
- GTTAACCCGT GAGTAGTTAG TGTTGTAAAA GGACAAGCTG CTACATCTGA CT - #GTGAGTTT
1560
- ATTCTCCAAA ATTTAGCAAT TAATTTTYCT TCTTCATTTA AAACGATTTC TG - #GTGAATTA
1620
- AAAAATTTCT CAATAAGTTG TGTTATCTCC AACGGTATTT CGTTTCATTT AA - #ACACACAT
1680
- CATTGAATAT ATATATATTA AAAATTAAGA TTAATATAAA TATTGTAATA TT - #TTTATTTT
1740
- TGATTTCCAT AATTAATTGT TTTTATAATT AAATTAGGTA AAGTAGTATC GA - #CGCCTAGT
1800
- AGTCCTAAAC ATATTATACC TCCACCTATT AATATTTTCT TTTTCAATTT TT - #TAGCGTGT
1860
- TCTTCACGTT CTTTTTGAAA AGTTTCTGCT CTCTCCTCTA TTCCTTGAAT AA - #AATTATTT
1920
- GTAATTTCTT CTAGTTCTTG AGAATTTTTG AGCTTTATTT CTTCTAAATA TT - #TATTAAAA
1980
- GTAGTTATTT GTTTATCTAA ATCGATTGAT ATTTGATTTG TGTTATAAAT AC - #ACATTGTT
2040
- TCACTTATCT TCTTCATAAA ATCTCTTACT AATAATCCCT CTATTTCTAA AT - #TCGATATC
2100
- GTATAAAGAA AAATGTTTCC TATTCGATAG AAATCTTCTT CAGTTATATT TG - #AATTAATT
2160
- GCTGTTCTTC TTAATAAATC ATTTATATAA GTTCTCACGT GAGGTGAGCT AT - #TTTCTATT
2220
- AATGATAAAA GATTTTCACT ATTATTTTCG TGATTTATAA TACTATTCAT AA - #TCTCTAAT
2280
- CTTCTTTCAG AAGATATGTG GTTATTTAAT TCAATAATTG TTTGAGAATC AA - #TTGATTCT
2340
- ATACCATTTA ACTTTTTTAT ATATGGTAAT TTATCTATAT TATTTAAAAG AT - #GATGATTT
2400
- ATCTTATCTC TAAAACTTTC CTGTAAATTA AAATTAGGAG GTTTTATTGG TG - #AACCTTTT
2460
- TCTTCAAATA ATAAGTTGCC TAATTTTAAG AAATCTTCTG ATTTAAAGTC TA - #TATTATTG
2520
- TTTATCATAT TTTATTTATT AAAAGACTTA AGAGTATTAT AAAATAATTT AA - #TACCTTCA
2580
- TCTAAAATAT CCCTGAAACG GATAATTCCT TCAGCCTCTG TTAATTGAAC TG - #TTGTAACA
2640
- GGGGATATTA CTGATCTTGC TACTAATCCA CTCACAATTT GAGGAACTCC TA - #TAGAAGTT
2700
- AAAGCCATTG ATCCTAATAT TCCATTTCGA TTTAAAGCTA TTTTCTGATC TA - #CTTCTCGA
2760
- TGAAATTCTT GAACGCGCTC ATCAATATGT TCCTCACTCG CTAACCTAAT CT - #CTTCTAAA
2820
- TATTGATTAT GGTTACTAAC TTGATTTTCA AGTATAGAGT AAATTTGATT TG - #TGTTAAAC
2880
- ATAACCATAG ATTCTCTCAT ATTTTGAATC ACATCTCTAA GAACTAATCC GT - #CTATATCT
2940
- AAATTGGATA TTGTATAAAG GAAAATGTTT CCTATTCTAT ATAAAACCTC TT - #CAGTTATA
3000
- TTTGAATTAT TTGCTGATCT AATTAATAAC TCGTGTAAAT AAGTCCTTAC TT - #CTGGTGAA
3060
- CTATGTTCAA TTAATAGAGC ACGATTTTCA TTATTATTTT CGTGATGTAT AA - #TACTATTC
3120
- ATAAATTCCA TTCTTCTTTC GGAAGTAGTT GAATTATTTA ATTCAATAAT TG - #TATTTGTA
3180
- TCAATCATAT CATTATTTCC TATATTATTA ATATAAAGTA AATTAGAAGT AT - #TTATTTCT
3240
- CTCAATTCTA CCATTAATAA TATTTTTTTT TAAATGTTCT ATAAAAGAAT TA - #AATTATAA
3300
- ACTTTTTTAA TTAAACAGTA GCTATAAAAA ATTCTTCAAT AGAGAAAGGT TT - #TATTTTTT
3360
- TAACAGAAAA TTGTAATCCT TATTCTACTT TAATAAATAA TCATAATATT TT - #AATAAGAA
3420
- ATAAATAATT AATATTTATA ATAAAATATA TTCTTATTAG AAGTATTTTC AT - #TTTAATTT
3480
- TTTTTTAAAA GTTATATATC TTTAAAAAGA TATAAATTAA TTACATAATA TG - #TTATTACA
3540
- ATCTGCAAAA TTTATTGGTG CTGGATTAGC TACTATTGGA TTAGCAGGTG CT - #GGTATCGG
3600
- TATCGGTTCA GTATTTAGTT CATTAGTTTT AGGTATTTCT AGAAACCCTT CT - #TTACAACA
3660
- AGATTTAACA AGAACAGCTA TTTTAGGTTT CGCTTTAACT GAATCTATTG CT - #TTATTCTG
3720
- TTTAATGATT GCTTTCTTAA TTTTATTCGC TTTTTAATTT AAGTTAATAA AA - #AATATTTT
3780
- TATTTCAATA CGAAATAGAA ATATTATTAA TTATATGTAT ACTTATAAAA TT - #AATCTATA
3840
- AAGATAATAG ATTAATTTTA TAAATAGATA TATCTCCATA TATTTTGAAA AA - #AACAATCA
3900
#       3933       AGCA GATTCAGCTG CAG
- (2) INFORMATION FOR SEQ ID NO:4:
-      (i) SEQUENCE CHARACTERISTICS:
#pairs    (A) LENGTH: 1218 base
          (B) TYPE: nucleic acid
          (C) STRANDEDNESS: single
          (D) TOPOLOGY: linear
-     (ii) MOLECULE TYPE: DNA (genomic)
-     (vi) ORIGINAL SOURCE:
#17-1     (C) INDIVIDUAL ISOLATE:
-     (xi) SEQUENCE DESCRIPTION: SEQ ID NO:4:
- CTGCAGCTGA ATCTGCTATA GGTTTAGCAA TAATGATTGT TTTTTTCAAA AT - #ATATGGAG
  60
- ATATATCTAT TTATAAAATT AATCTATTAT CTTTATAGAT TAATTTTATA AG - #TATACATA
 120
- TAATTAATAA TATTTCTATT TCGTATTGAA ATAAAAATAT TTTTTATTAA CT - #TAAATTAA
 180
- AAAGCGAATA AAATTAAGAA AGCAATCATT AAACAGAATA AAGCAATAGA TT - #CAGTTAAA
 240
- GCGAAACCTA AAATAGCTGT TCTTGTTAAA TCTTGTTGTA AAGAAGGGTT TC - #TAGAAATA
 300
- CCTAAAACTA ATGAACTAAA TACTGAACCG ATACCGATAC CAGCACCTGC TA - #ATCCAATA
 360
- GTAGCTAATC CAGCACCAAT AAATTTTGCA GATTGTAATA ACATATTATG TA - #ATTAATTT
 420
- ATATCTTTTT AAAGATATAT AACTTTTAAA AAAAAATTAA AATGAAAATA CT - #TCTAATAA
 480
- GAATATATTT TATTATAAAT ATTAATTATT TAAATTGTGT AAATCCACCA GA - #AATTTTAA
 540
- CTATTATAAA TATTGAAGAA CTTTTACTTA TATTTCTAAA TAATAATCTG AA - #TTTAAACA
 600
- GTAGACCCTA TGAACCTTTA ATAATAGCTA TAAGAAATTT TTCAATAGAG AA - #AGGTTTTA
 660
- TTTTTTTAAT AGAAAATTGT AATTCTTATT TTACTTTAAT AAGAAATAAA TA - #ATTAATAT
 720
- TTATAATAAA ATATATTCTT ATTAGAAGTA TTTTCATTTT AATTTTTTTT TA - #AAAGTTAT
 780
- ATATCTTTAA AAAGATATAA ATTAATTACA TAATATGTTA TTACAATCTG CA - #AAATTTAT
 840
- TGGTGCTGGA TTAGCTACTA TTGGATTAGC AGGTGCTGGT ATCGGTATCG GT - #TCAGTATT
 900
- TAGTTCATTA GTTTTAGGTA TTTCTAGAAA CCCTTCTTTA CAACAAGATT TA - #ACAAGAAC
 960
- AGCTATTTTA GGTTTCGCTT TAACTGAATC TATTGCTTTA TTCTGTTTAA TG - #ATTGCTTT
1020
- CTTAATTTTA TTCGCTTTTT AATTTAAGTT AATAAAAAAT ATTTTTATTT CA - #ATACGAAA
1080
- TAGAAATATT ATTAATTATA TGTATACTTA TAAAATTAAT CTATAAAGAT AA - #TAGATTAA
1140
- TTTTATAAAT AGATATATCT CCATATATTT TGAAAAAAAC AATCATTATT GC - #TAAACCTA
1200
#1218              AG
- (2) INFORMATION FOR SEQ ID NO:5:
-      (i) SEQUENCE CHARACTERISTICS:
#pairs    (A) LENGTH: 1186 base
          (B) TYPE: nucleic acid
          (C) STRANDEDNESS: single
          (D) TOPOLOGY: linear
-     (ii) MOLECULE TYPE: DNA (genomic)
-     (vi) ORIGINAL SOURCE:
#23-5     (C) INDIVIDUAL ISOLATE:
-     (xi) SEQUENCE DESCRIPTION: SEQ ID NO:5:
- CTGCAGCTGA ATCTGCTATA GGTTTAGCAA TAATGATTGT TTTTTTCAAA AT - #ATATGGAG
  60
- ATATATCTAT TTATAAAATT AATCTATTAT CTTTATAGAT TAATTTTATA AG - #TATACATA
 120
- TAATTAATAA TATTTCTATT TCGTATTGAA ATAAAAATAT TTTTTATTAA CT - #TAAATTAA
 180
- AAAGCGAATA AAATTAAGAA AGCAATCATT AAACAGAATA AAGCAATAGA TT - #CAGTTAAA
 240
- GCGAAACCTA AAATAGCTGT TCTTGTTAAA TCTTGTTGTA AAGAAGGGTT TC - #TAGAAATA
 300
- CCTAAACTAA TGAACTAAAT ACTGAACCGA TACCGATACC AGCACCTGCT AA - #TCCAATAG
 360
- TAGCTAATCC AGCACCAATA AATTTTGCAG ATTGTAATAA CATATTATGT AA - #TTAATTTA
 420
- TATCTTTTTA AAGATATATA ACTTTTAAAA AAAAATTAAA ATGAAAATAC TT - #CTAATAAG
 480
- AATATATTTT ATTATAAATA TTGAAAAACT TTTATTTATA TTTTTAAATA AT - #GATCTGGA
 540
- TTTATACAGT AGATCCTATA AATCTTTAAT AGTAGTTATA AGAAATTCTT CA - #ATAGAGAA
 600
- AGGTTTTATT TTTTCAATAG AAAATTGTAA TTCTTATTCT ATTTTAATAA AT - #AATCGTAA
 660
- TACTTTAATA AGAAATAAAT AATTAATATT TATAATAAAA TATATTCTTA TT - #AGAAGTAT
 720
- TTTCATTTTA ATTTTTTTTT AAAAGTTATA TATCTTTAAA AAGATATAAA TT - #AATTACAT
 780
- AATATGTTAT TACAATCTGC AAAATTTATT GGTGCTGGAT TAGCTACTAT TG - #GATTAGCA
 840
- GGTGCTGGTA TCGGTATCGG TTCAGTATTT AGTTCATTAG TTTAGGTATT TC - #TAGAAACC
 900
- CTTCTTTACA ACAAGATTTA ACAAGAACAG CTATTTTAGG TTTCGCTTTA AC - #TGAATCTA
 960
- TTGCTTTATT CTGTTTAATG ATTGCTTTCT TAATTTTATT CGCTTTTTAA TT - #TAAGTTAA
1020
- TAAAAAATAT TTTTATTTCA ATACGAAATA GAAATATTAT TAATTATATG TA - #TACTTATA
1080
- AAATTAATCT ATAAAGATAA TAGATTAATT TTATAAATAG ATATATCTCC AT - #ATATTTTG
1140
#               1186TGC TAAACCTATA GCAGATTCAG CTGCAG
- (2) INFORMATION FOR SEQ ID NO:6:
-      (i) SEQUENCE CHARACTERISTICS:
#pairs    (A) LENGTH: 934 base
          (B) TYPE: nucleic acid
          (C) STRANDEDNESS: single
          (D) TOPOLOGY: linear
-     (ii) MOLECULE TYPE: DNA (genomic)
-     (vi) ORIGINAL SOURCE:
#1986-42  (C) INDIVIDUAL ISOLATE:
-     (xi) SEQUENCE DESCRIPTION: SEQ ID NO:6:
- TGCAGCTGAA TCTGCTATAG GTTTAGCAAT AATGATTGTT TTTTTCAAAA TA - #TATGGAGA
  60
- TATATCTATT TATAAAATTA ATCTATTATC TTTATAGATT AATTTTATAA GT - #ATACATAT
 120
- AATTAATAAT ATTTCTATTT CGTATTGAAA TAAAAATATT TTTTATTAAC TT - #AAATTAAA
 180
- AAGCGAATAA AATTAAGAAA GCAATCATTA AACAGAATAA AGCAATAGAT TC - #AGTTAAAG
 240
- CGAAACCTAA AATAGCTGTT CTTGTTAAAT CTTGTTGTAA AGAAGGGTTT CT - #AGAAATAC
 300
- CTAAAACTAA TGAACTAAAT ACTGAACCGA TACCGATACC AGCACCTGCT AA - #TCCAATAG
 360
- TAGCTAATCC AGCACCAATA AATTTTGCAG ATTGTAATAA CATATTATGT AA - #TTAATTTA
 420
- TATCTTTTTA AAGATATATA ACTTTTAAAA AAAAAATTAA AATGAAAATA CT - #TCTAATAA
 480
- GAATATATTT TATTATAAAT ATTGAAAAAC TTTTACTTAT ATTTTTAAAT AA - #TGATCTGG
 540
- ATTTAGACAG TAGATCCTAT AAACCTTTAA TAGTAATTAT AAGAAATTCT TC - #AATAGAGA
 600
- AAGGTTTTAT TTTTTCAATA GAAAATTGTA ATTCTTATTC TACTTTAATA AA - #CAATCATA
 660
- ATACTTTAAT AAGAACAGCT ATTTTAGGTT TCGCTTTAAC TGAATCTATT GC - #TTTATTCT
 720
- GTTTAATGAT TGCTTTCTTA ATTTTATTCG CTTTTTAATT TAAGTTAATA AA - #AAATATTT
 780
- TTATTTCAAT ACGAAATAGA AATATTATTA ATTATATGTA TACTTATAAA AT - #TAATCTAT
 840
- AAAGATAATA GATTAATTTT ATAAATAGAT ATATCTCCAT ATATTTTGAA AA - #AAACAATC
 900
#       934        TAGC AGATTCAGCT GCAG
- (2) INFORMATION FOR SEQ ID NO:7:
-      (i) SEQUENCE CHARACTERISTICS:
#pairs    (A) LENGTH: 565 base
          (B) TYPE: nucleic acid
          (C) STRANDEDNESS: single
          (D) TOPOLOGY: linear
-     (ii) MOLECULE TYPE: DNA (genomic)
-     (vi) ORIGINAL SOURCE:
#27-6     (C) INDIVIDUAL ISOLATE:
-     (xi) SEQUENCE DESCRIPTION: SEQ ID NO:7:
- CTGCAGCTGA ATCTGCTATA GGTTTAGCAA TAATGATTGT TTTTTTCAAA AT - #ATATGGAG
  60
- ATATATCTAT TTATAAAATT AATCTATTAT CTTTATAGAT TAATTTTATA AG - #TATACATA
 120
- TAATTAATAA TATTTCTATT TCGTATTGAA ATAAAAATAT TTTTTATTAA CT - #TAAATTAA
 180
- AAAGCGAATA AAATTAAGAA AGCAATCATT AAACAGAATA AAGCAATAGA TT - #CAGTTAAA
 240
- GCGAAACCTA AAATAGCTGT TCTTGTTAAA TCTTGTTGTA AAGAAGGGTT TC - #TAGAAATA
 300
- CCTAAACTAA TGAACTAAAT ACTGAACCGA TACCGATACC AGCACCTGCT AA - #TCCAATAG
 360
- TAGCTAATCC AGCACCAATA AATTTTGCAG ATTGTAATAA CATATTATGT AA - #TTAATTTA
 420
- TATCTTTTTA AAGATATATA ACTTTTAAAA AAAAAATTAA AATGAAAATA CT - #TCTAATAA
 480
- GAATATATTT TATTATAAAT ATTGAAAAAC CTTTACTTAT ATTTTTAAAT AA - #TGATCTGG
 540
#              565 CTAT AAACC
- (2) INFORMATION FOR SEQ ID NO:8:
-      (i) SEQUENCE CHARACTERISTICS:
#pairs    (A) LENGTH: 1183 base
          (B) TYPE: nucleic acid
          (C) STRANDEDNESS: single
          (D) TOPOLOGY: linear
-     (ii) MOLECULE TYPE: DNA (genomic)
-     (vi) ORIGINAL SOURCE:
#30-1     (C) INDIVIDUAL ISOLATE:
-     (xi) SEQUENCE DESCRIPTION: SEQ ID NO:8:
- CTGCAGCTGA ATCTGCTATA GGTTTAGCAA TAATGATTGT TTTTTTCAAA AT - #ATATGGAG
  60
- ATATATCTAT TTATAAAATT AATCTATTAT CTTTATAGAT TAATTTTATA AG - #TATACATA
 120
- TAATTAATAA TATTTCTATT TCGTATTGAA ATAAAAATAT TTTTTATTAA CT - #TAAATTAA
 180
- AAAGCGAATA AAATTAAGAA AGCAATCATT AAACAGAATA AAGCAATAGA TT - #CAGTTAAA
 240
- GCGAAACCTA AAATAGCTGT TCTTGTTAAA TCTTGTTGTA AAGAAGGGTT TC - #TAGAAATA
 300
- CCTAAACTAA TGAACTAAAT ACTGAACCGA TACCGATACC AGCACCTGCT AA - #TCCAATAG
 360
- TAGCTAATCC AGCACCAATA AATTTTGCAG ATTGTAATAA CATATTATGT AA - #TTAATTTA
 420
- TATCTTTTTA AAGATATATA ACTTTTAAAA AAAAAATTAA AATGAAAATA CT - #TCTAATAA
 480
- GAATATATTT TATTATAAAT ATTAATTATT TAAATTATAC AAATCCATCA GA - #AATTTTAA
 540
- CTGTTATAAA TATTAAAGAA CCTTTACTTA TATTTCTAAA TAATGACTGA AT - #TTAAACAG
 600
- TAGACCTTAT GNNNNNNNNN NNNNNNNNNN NNNNNNNNNN NNNNNNNNNN NN - #NNNNNNNN
 660
- NNNNNNNNNN NTAAATAATT AATATTTATA ATAAAATATA TTCTTATTAG AA - #GTATTTTC
 720
- ATTTTAATTT TTTTTTTAAA AGTTATATAT CTTTAAAAAG ATATAAATTA AT - #TACATAAT
 780
- ATGTTATTAC AATCTGCAAA ATTTATTGGT GCTGGATTAG CTACTATTGG AT - #TAGCAGGT
 840
- GCTGGTATCG GTATCGGTTC AGTATTTAGT TCATTAGTTT AGGTATTTCT AG - #AAACCCTT
 900
- CTTTACAACA AGATTTAACA AGAACAGCTA TTTTAGGTTT CGCTTTAACT GA - #ATCTATTG
 960
- CTTTATTCTG TTTAATGATT GCTTTCTTAA TTTTATTCGC TTTTTAATTT AA - #GTTAATAA
1020
- AAAATATTTT TATTTCAATA CGAAATAGAA ATATTATTAA TTATATGTAT AC - #TTATAAAA
1080
- TTAATCTATA AAGATAATAG ATTAATTTTA TAAATAGATA TATCTCCATA TA - #TTTTGAAA
1140
#                 118 - #3CTATAGCA GATTCAGCTG CAG
__________________________________________________________________________

Claims (16)

I claim:
1. A method for controlling a fungal infestation in a plant comprising contacting said plant with an effective amount of a non-phytopathogenic Pythium oligandrum isolate selected from the group consisting of isolate 70-1 (ATCC 74395), isolate 25-6 (ATCC 74393) and isolate 30-1 (ATCC 74394).
2. The method, according to claim 1, wherein said fungus is a Pythium species.
3. The method, according to claim 1, wherein said method further comprises contacting said fungus with an agriculturally acceptable fungicide.
4. The method, according to claim 1, wherein said non-phytopathogenic organism has the characteristic of having activity at low-level root colonization wherein low-level root colonization is under 3 colonies recovered per centimeter of root.
5. The method, according to claim 4, wherein said low-level root colonization is approximately 0.1 colonies recovered per centimeter of root.
6. A method for protecting a plant from damping-off comprising administering an effective amount of a non-phytopathogenic Pythium oligandrum isolate selected from the group consisting of isolate 70-1 (ATCC 74395), isolate 25-6 (ATCC 74393) and isolate 30-1 (ATCC 74394) to said plant.
7. The method, according to claim 6, wherein said damping-off is caused by a phytopathogenic fungus.
8. The method, according to claim 7, wherein said phytopathogenic fungus is a Pythium species.
9. The method, according to claim 7, wherein said plant is a tomato plant.
10. The method, according to claim 6, wherein said plant to be protected is a potted seedling or transplant.
11. The method, according to claim 10, wherein said plant is a vegetable crop.
12. The method, according to claim 6, wherein the situs of the plant is soil surrounding roots of the plant.
13. The method, according to claim 12, wherein the soil is in a transplant pot.
14. A biologically pure non-phytopathogenic Pythium oligandrum isolate selected from the group consisting of isolate 70-1 (ATCC 74395), isolate 25-6 (ATCC 74393) and isolate 30-1 (ATCC 74394).
15. The isolate of claim 14, wherein said isolate is mycotoxic.
16. The isolate of claim 14, wherein the isolate is 70-1 (ATCC 74395).
US08/731,722 1996-10-17 1996-10-17 Biocontrol of fungal soilborne pathogens by Pythium oligandrum Expired - Fee Related US5961971A (en)

Priority Applications (3)

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US08/731,722 US5961971A (en) 1996-10-17 1996-10-17 Biocontrol of fungal soilborne pathogens by Pythium oligandrum
AU48154/97A AU4815497A (en) 1996-10-17 1997-10-10 Biocontrol of fungal soilborne pathogens by (pythium oligandrum)
PCT/US1997/018343 WO1998016110A1 (en) 1996-10-17 1997-10-10 BIOCONTROL OF FUNGAL SOILBORNE PATHOGENS BY $i(PYTHIUM OLIGANDRUM)

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US20130035230A1 (en) * 2009-11-27 2013-02-07 Suchanek Martin Use of fungal organism pythium oligandrum
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